key: cord-0035218-ho8k9qji authors: Okafor, Nduka title: Taxonomy, Physiology, and Ecology of Aquatic Microorganisms date: 2011-03-04 journal: Environmental Microbiology of Aquatic and Waste Systems DOI: 10.1007/978-94-007-1460-1_4 sha: 50083c2cd1cea4b144609af991ab31ddba4a995d doc_id: 35218 cord_uid: ho8k9qji The principles behind the taxonomy of the microorganisms, especially the ­molecular approach (using the sequence of the 16S RNA in the small subunit of the ribosome) in the identification of bacteria, are discussed. The detailed taxonomy of bacteria, fungi, algae, protozoa, and viruses (including bacteriophages) is discussed, and emphasis is laid on those microorganisms which are aquatic. The chapter includes information on some of the smaller macroorganisms found in water such as nematodes and rotifers. The activities of aquatic microorganisms in photosynthesis, and the global cycling of nitrogen and sulfur is discussed. Taxonomy is important because it: 1. Allows the orderly organization of huge amounts of information regarding organisms 2. Enables predictions about their properties and formation of hypothesis about them 3. Facilitates the accurate characterization and identification of "unknown" organisms 4. Places organisms in meaningful manageable groups and thus facilitates scientific communication Landmarks in the evolution and development of bio logical classification may be ascribed to the contribu tions of the following: 1. Linnaeus The Swedish naturalist, Carolus Linnaeus, is credited with introducing the earliest organized classification of living things in his Systema Naturae or natural system. He divided living things into plants and ani mals. Based on morphology and motility, the dis tinction between the two groups of organisms was clear: plants were green and did not move; on the other hand, animals were not green, but moved. Soon after the discovery of the microscope, previ ously invisible microscopic organisms were observed, some of which had properties common to both plants and animals. Some such as Euglena were green like, but they also moved about like animals. Because the clearcut criteria which separated plants from animals were absent in these "new" organisms, the German biologist who was a contemporary of Charles Darwin, in 1866 coined the name Protista for a third kingdom, in addition to the Plant and Animal Kingdoms. 3. Robert Harding Whittaker (1920 -1980 Whittaker was an American. Born in Wichita, Kansas, he worked in various places including the University of California, Irvine, and Cornell University. In 1968, he proposed the fivekingdom taxonomic classifica tion of living things into the Animalia, Plantae, Fungi, Protista (Algae and Protozoa), and Monera (Bacteria). His categorization of living things was based on three criteria: celltype (whether prokaryotic or eukaryotic); organizational level (unicellular or multicellular); nutritional type (autotrophy or heterotrophy). 4. Carl R. Woese (1928-) The current classification of living things is based on the work of Carl Robert Woese of the University of Illinois. While earlier classifications were based mainly on morphological characteristics and cell type, following our greater understanding of living things at the molecular level, Woese's classification is based on the sequence of the gene of the ribosomal RNA (rRNA) in the 16S of the small subunit of the prokaryotic ribosome, or the 18S of the small subunit of the eukaryotic ribosome (Petti et al. 2006) . The sequence of the rRNA in the 16S or 18S of the small subunit of the ribosome is used for the following reasons: (a) The ribosome is an important organelle in all living things where it is used for a basic function for the support of life, namely, protein synthesis. From parent to offspring (vertical gene transfer), or by horizontal or lateral gene transfer, in which genes jump between unrelated organisms, a common phenomenon in prokaryotes. There is little or no lateral gene transfer in the sequences in the 16S or 18 S RNA of the ribosomal small units. All the above properties make the sequence of the rRNA in the 16S or 18S of the small subunit of the ribosome useful as molecular chronometers for mea suring evolutionary changes among organisms. Using this method, living things are now divided into three domains: Archae, Bacteria, and Eukarya. A diagram matic representation of the three domains is given in Fig. 4 .1, and their distinguishing properties are given in Table 4 .1 (Woese 1987 (Woese , 2000 (Woese , 2002 . The smallest unit of biological classification is the Initiator tRNA Formylmethionine Methionine Methionine 9. Introns in most genes b − − + 10. Operons c + + − 11. Plasmids + + Rare 12. Ribosome sensitive to diphtheria toxin − + + 13. Sensitivity to streptomycin, chloramphenicol, and kanamycin + − − Physiological/special structures 14. Methanogenesis + + − 15. Denitrification + + − 16. Nitrogen fixation + + − 17. Chlorophyllbased photosynthesis + -+ (Plants) 18. Gas vesicles + + − 19. Chemolithotrophy + + − 20. Storage granules of polybhydroxyalkanoates + + − 21. Growth above 80°C + + − 22. Growth above 100°C − + − a Histone proteins are present in eukaryotic chromosomes; histones and DNA give structure to chromosomes in eukaryotes; proteins in archeae chromosomes are different b Noncoding sequences within genes c Operons: Typically present in prokaryotes, these are clusters of genes controlled by a single operator d TATA box (also called Hogness Box): an ATrich region of the DNA with the sequence TATAT/AAT/A located before the initiation site e Transcription factor is a protein that binds DNA at a specific promoter or enhancer region or site, where it regulates transcription Several mnemonics exist to help with remembering the correct order of the listing of taxonomic groups. Two are given below: Biological objects, including microorganisms are named in the binomial system devised by Carolus Linnaeus. The genus name is written first and begins with an uppercase (capital) letter; the other half of the name is written in lowercase (small) letters and is the species name. The two are written in italics or underlined if written in long hand. When written for mally, the name of the author who first described the organism is included and the year of the publication is given; the names are usually written in Latin or lati nized. The name of a hypothetical Bacillus discovered in water by John Smith and published in 2007 could be Bacillus aquanensis Smith 2007. Usually only the genus and species names are given; the author and year of publication are omitted (van Regenmortel 1999) . Whereas members of the Domain Eukarya are classified largely on their morphological characteristics which are adequately diverse, morphological types are very lim ited in the Domains Bacteria and Archae. Therefore, while morphological properties are used, other charac teristics are employed in addition to morphology. The properties used for classifying and identifying unknowns among organisms in the Domains Bacteria and Archae are given in Table 4 .3. The principles of methods used are described briefly below. Living things are classified into major nutritional types on the basis of the following attributes: (a) Carbon source utilized A carbon skeleton is required for the compounds used for growth and development such as carbo hydrates, amino acids, fats, etc. The organism is autotrophic if it manufactures its food and obtains its carbon through fixing CO 2 such as is the case with plants, algae, and some bacteria. When the organism cannot manufacture its own food from CO 2 but must utilize food already manufactured from CO 2 , in the form of carbo hydrates, proteins etc., it is heterotrophic. This is the case with animals and most bacteria. Energy release (i) Lithotrophy (ii) Organotrophy 3. Cell wall: Gram reaction (i) Gram negative (ii) Gram positive 4. Cell morphology (i) Cell shapes (ii) Cell aggregation (iii) Flagellation -motility (iv) Spore formation and location (v) Special staining, e.g., Ziehl-Nielsen 5. Physiological properties (i) Utilization of various sugars (ii) Utilization of various polysaccharides (iii) Utilization of various nitrogenous substrates (iv) Oxygen requirement (v) Temperature requirements (vi) pH requirement (vii) Production of special enzymes, e.g., catalase, coagulase, optochin, oxidase 6. Antigenic properties 7. Molecular (nucleic acid) methods (i) G + C composition (ii) DNA:DNA hybridization (iii) Ribotyping (iv) Fluorescent insitu hybridization (FISH) 8. Chemical analysis (Chemotaxonomy) (i) Lipid analysis (ii) Protein analysis (b) Source of reducing equivalent During the generation of energy in the cell, electrons are transferred from one compound to another. An organism is said to be organ otrophic when it uses organic compounds as a source of electrons. When the source of elec trons is inorganic, it is said to be lithotrophic. (c) Source of energy Some organisms derive energy for the genera tion of ATP used for the biosynthesis of new compounds and other cellular activities from sunlight; such organisms are phototrophic. When the generation of ATP occurs through energy obtained from chemical reactions, the organism is said to be chemotrophic. The carbon source utilized, the source of reducing equivalent, and the source of energy determine the nutritional type of bacteria, and a wide variety of combinations of these three is possible. Table 4 .4 gives a selection of the possible permutations. The Gram stain was devised by the German doctor, Christian Gram in 1884 and divides bacteria into two groups: Gram positive and Gram negative. On account of the greater thickness of peptidoglycan in the Gram positive wall (see Fig. 4 .2), the iodine crystal violet stain in the Gram stain is retained when decolorized with dilute acid, whereas it is removed in the Gram negative cell wall. The Gram stain also divides all bacteria into two groups regarding their susceptibility to the classical antibiotic penicillin: Grampositive bacteria, being susceptible, while Gram negative bacteria are not ( Fig. 4.3 ). (a) Individual cell shapes Cell shapes in bacteria are limited and are spheres (coccus-cocci, plural), rods, spiral, or comma or vibrio (see Fig. 4 .4). The flagella may be at one end (polar) and may occur singly or as a tuft. The flagella may occur all around the cell when it is peritrichous (see Fig. 4 .5). Spores are bodies resistant to heat and other adverse conditions which may be terminal or placed midway in the cell; in either position, it may be less than the diameter of the cell or may be wider. The terminal wider spore gives the shape of a drumstick, and is diagnostic of the anaerobic rodlike sporeformer, Clostridium tet anii, the causative agent of tetanus (see Fig. 4 .6). If the bacterium is suspected to belong to Myco bacterium spp., or any of the other acidfast bacteria it might be stained with hot basic fuchsin; acid fast bacteria retain the dye when decolorized. Utilization of various sugars, carbohydrates, and nitrogenous sources The ability of the organism to produce acid and/or gas from a medium containing a particular substrate is diagnostic of its ability to utilize it. The utilization of a wide range of sugars and other carbohydrates, and nitrogen sources including urea is tested by the pres ence of gas in the small (Durham) tube placed in the Note that the peptidoglycan layer is very thick in Gram +ve walls, but very thin in Gram -ve bacterial cells. This thick peptidoglycan enables Gram +ve walls retain crystal violet, the primary stain in the Gram, when decolorized with dilute acid. Crystal violet is not retained in Gram -ve bacteria because the peptidoglycan layer is thin. The Gram -ve wall would be color less after decolorization with dilute acid. However in the Gram stain, after decolourization, the cells are counterstained with a red stain, safranin. On account of this the Gram negative cells appear red in the Gram stain, while Gram +ve cells are violet (see text and Fig. 4 .3) test tube containing the medium; a change in the color of indicator would indicate acid production by the organism (see Fig. 4.7) . Optimum pH, temperature, and oxygen requirements are determined by growing the organism under dif ferent conditions of pH and temperature and finding the best condition. For oxygen requirement, the organism may be grown in an agar stab and sealed with sterile molten petroleum jelly to determine if it will grow under anaerobic conditions. 6. Secretion of special enzymes The secretion of unique enzymes is diagnostic. Some of the following enzymes are diagnostic (see Fig. 4 .7a). In microbiology, the catalase test is used to differenti ate between staphylococci and micrococci, which are catalasepositive, from streptococci and enterococci, which are catalasenegative Optochin: Optochin (ethyl hydrocuprein hydro chloride) is used for the presumptive identification of Streptococcus pneumoniae, which is optochin sensitive, from Streptococcus viridans which is resistant. Bacteria that are optochin sensitive will not continue to grow (i.e., Streptococcus pneumo niae will die), while bacteria that are not optochin sensitive will be unaffected (i.e., Streptococcus viridans will survive). Oxidase: An oxidase is any enzyme that catalyzes an oxidation/reduction reaction involving molecular oxy gen (O 2 ) as the electron acceptor. In these reactions, oxygen is reduced to water (H 2 O) or hydrogen perox ide (H 2 O 2 ). The oxidases are a subclass of the oxi doreductases. In microbiology, the oxidase test is used as a phenotypic character for the identification of bac terial strains; it determines whether a given bacterium produces cytochrome oxidases (and therefore utilizes oxygen with an electron transfer chain) (see Fig. 4 .7a). Bacterial species and serotypes can be identified by specific antigen/antibody reactions. Antigens are substances that induce the production of antibodies in an animal body. Bacteria and bacterial components serve as excellent antigens. The test includes production of antibodies in an animal host and test ing of the antiserum by either the agglutination or precipitation test. In the agglutination test, a drop of the culture of a particular bacterium is mixed on a slide with the antiserum of an individual infected by it and examined under a microscope. If clump ing occurs, the test bacterium is considered to be the same or closely related to the bacterium used as the antigen. The methods for the characterization and identification of bacteria which have been discussed so far are based on phenotypic properties, i.e., the outward manifesta tion of the innate (genetic) attributes of the organism. The properties to be discussed in this section are those of the nucleic acids of the organisms. They alone how ever do not define the organism and must be taken along with the phenotypic properties. They are very useful in refining the description of an organism. They are par ticularly useful in identifying strains within a species. (a) G + C ratio The G + C ratio is the percentage of guanine + cyto sine in an organism's DNA. Several methods exist for determining this ratio. One method is to deter mine the Tm or temperature of melting of the DNA. At room temperature, DNA is double stranded. However, as its temperature is raised gradually, the two strands separate and the rapidity of separa tion with increasing temperature depends on the amount of G and C in the organism's DNA. G and C are linked by triple bonds and are therefore less likely to separate than A and T bonds, which have double bonds. The higher the G + C content, the higher the temperature at which the DNA separates completely. DNA begins to separate at 70-75°C and separates completely at about 90°C, when it is said to have melted. When cooled slowly, it begins to anneal (i.e., to reform itself into double strands). In anneal ing, the strands do not return to their previous " partners" but will anneal with any strand with com plimentary bases no matter the source, including those coming from the same organism, other orga nisms, or even those synthesized in the laboratory. This phenomenon of annealing with complimentary strands from any source is important in other proce dures such as in the identification of unknowns, the Polymerase Chain Reaction (PCR), etc. When the Tm method is used to determine the G + C composition, the temperature of the double (ds) DNA is raised slowly and subjected to spectro photometric reading at 260 nm. The graph of the spectrophotometric readings is plotted against the change in temperature (see Fig. 4 .8). The Tm is the midpoint of the resulting graph. Two organisms with similar phenotypic properties and the same G + C ratio are likely to belong to the species. This technique measures the degree of genetic similarity between pools of DNA sequences. It is usually used to determine the genetic distance between two species. It was seen above that when melted DNA is allowed to cool slowly, the singlestranded DNA will anneal with any singlestranded DNA no matter its source, as long the bases are complimen tary. To determine how closely related an unknown organism is with a known one, DNA from the two organisms are mixed and heated slowly and allowed to anneal slowly. The unknown or the known is labeled with a fluorescent dye or with radioactive phosphorous and measured at 260 nm in the spectrophotometer. The extent of the taxonomic relatedness is reflected in the extent of the annealing. If the two organisms are of the same species, there will be complete annealment. Some authors have suggested that organisms of the same species will have 90% annealing, while those of the same genus will have about 75% annealing. Ribotyping is an RNAbased molecular character ization of bacteria. In ribotyping, bacteria genomic DNAs are digested and separated by gel electro phoresis. Universal probes that target specific con served domains of ribosomal RNA coding sequences are used to detect the band patterns. Ribosomal genes are known to be highly con served in microbes, meaning that the genetic infor mation coding for rRNA will vary much less within bacteria of the same strain than it will between bacterial strains. This characteristic allows for a greater ability to distinguish between different bacterial strains. In ribotyping, restriction enzymes (i.e., enzymes which cut DNA at specific positions) are used to cut the genes coding for rRNA into pieces, and gel electrophoresis is used to separate the pieces by size. Genetic probes then visualize locations of differentsize fragments of DNA in the gel, which appear as bands. The banding pattern of DNA fragments corresponding to the relevant rRNA is known as the ribotype. A probe is a strand of nucleic acid which is synthesized in the laboratory and can be labeled with a dye or radioactively. Probes are used to hybridize to a complementary nucleic acid from a mixture. Probes can be general or specific. Thus, it is possible to design probes which will bind to sequences in the ribosomal RNA of all organisms irrespective of Domain. On the other hand, specific probes can be designed which will react only with nucleic acid of Bacteria, Archae, or Eukarya because of the unique sequences found in these groups. Even within species in the various domains, signature sequences exist which will enable the identification of the species using probes (see Table 4 .5). Ribotyping is so specific that it has been nicknamed "molecular finger printing." This is a special type of ribotyping. In FISH, the whole organism is used without need to isolate the organism's DNA. The cells are treated with chem icals which make the cell walls and cell mem branes permeable, thus permitting the entry of probes labeled with fluorescent dyes. After hybrid ization of the ribosomes with the dye, the entire organism fluoresces and can be seen under the light microscope. FISH is widely used in ecologi cal and clinical studies. It can be used for the rapid identification of bacterial pathogens in clinical specimens; ordinary procedures take about 48 h, but FISH can be completed in a few hours. Proteins are isolated from the whole bacterium, the cell membrane, or the ribosome. The proteins are run in a twodimensional gel electrophoresis on polyacrylamide gel. The first run separates the proteins on the basis of their molecular weights and the second on the basis of their isoelectric points (Ochiai and Kawamoto 1995) . The result ing protein pattern is diagnostic of a particular organism. If many samples are examined, the (FAME) This method is widely used in clinical, food, and water microbiology for the identification of bacte ria. Fatty acids from the cell membrane of bacteria as well from the outer membrane of Gram negative bacteria are extracted and converted to their methyl esters. The esters are then run in a gas chromato graph. The patterns of the gas chromatograms are diagnostic and can be used to identify unknowns. For example, Burkholderia pseudomallei, the cause of melioidosis, has been distinguished from the closely related but nonpathogenic Burkholderia thailandensis by gas chromatography (GC) analy sis of fatty acid derivatives. A 2-hydroxymyristic acid derivative (14:0 2OH) was present in 95% of B. pseudomallei isolates but absent from all B. thailandensis isolates (see Table 4 .6) (Inglis et al. 2003; Banowetz et al. 2006 Garrity 2001 Garrity -2006 . The manuals are named after Dr. D H Bergey who was the first Chairman of the Board set up by the then Society of American Bacteriologists (now American Society for Microbiology) to publish the books. The publication of Bergey Manuals is now managed by the Bergey's Manual Trust. Of the 18 phyla in the bacteria (see Figs. 4.9 and 4.10), the Aquiflex is evolutionarily the most primitive, while the most advanced is the Proteobacteria. In the following discussion, emphasis will be laid on the bacteria which are aquatic. 1. Aquifex The two species generally classified in Aquifex are A. pyrophilus and A. aeolicus. Both are highly ther mophilic, growing best in water temperature of 85-95°C. They are among the most thermophilic bacteria known. They can grow on hydrogen, oxy gen, carbon dioxide, SO 2 , S 2 O 3, or NO 3 and mineral salts, functioning as a chemolithoautotroph (an organism which uses an inorganic carbon source for biosynthesis and an inorganic chemical energy source). As a hyperthermophilic bacterium, Aquifex aeolicus grows in extremely hot tempuratures such as near volcanoes or hot springs. They grow opti mally at temperatures around 85°C but can grow at temperatures up to 95°C. It needs oxygen to carry on its metabolic machinery, but it can function in relatively low levels of oxygen. The genus Aquifex consists of Gram negative rods. 2. Thermodesulfobacterium Thermodesulfobacterium is a thermophilic sulfate reducer. Sulfate reducers include a wide range of morphological types, including rods, vibrios, ovals, spheres, and even teardropped or onion shaped cells. Some are motile, others are not. Most sulfatereducing bacteria are mesophilic, but a few are thermophiles, among which is the Gram nega tive and anaerobic Thermodesulfobacterium. The bacterium is nonsporeforming. It is an aquatic organism and has been isolated from volcanic hot springs, deepsea hydrothermal sulfides, and other marine environments. In marine sediments and in aerobic wastewater treatment systems, sulfate reduction accounts for up to 50% of the mineral ization of organic matter. Furthermore, sulfate reduction strongly stimulates microbially enhanced corrosion of metals. Sulfate Reducing Bacteria (SRB) are discussed in more detail later. Thermotoga is typically a rodshaped cell envel oped in an outer cell membrane (the "toga" or jacket). Thermotoga enzymes are known for being active at high temperatures. Enzymes from Thermotoga spp. are extremely thermostable and therefore, useful for many industrial processes such as in the chemical and food industries. The organisms are thermophilic or hyperthermophilic, growing best around 80°C and in the neutral pH range. The salt tolerance of Thermotoga species varies greatly; while some display an extremely high salt tolerance, others are restricted to low salinity habitats. This aerobic Gramnegative organism is typically nonsporeforming and metabolizes several carbohydrates, both simple and complex, including glucose, sucrose, starch, cellulose, and xylan. It can grow by anaerobic res piration using H 2 as electron donor and Fe 3+ as electron acceptor. It is found in hot springs and in the hydrothermic vents of ocean floors. Thermotoga maritime has been widely studied. The Green nonsulfur bacteria are now known as Chloroflexi are typically filamentous, and can move about by bacterial gliding. They are facultatively aerobic and have a different method of carbon fixa tion (photoheterotrophy) from other photosynthetic bacteria. Like green plants, they also carry out pho tosynthesis, but there are differences between the two; for instance, unlike plants, they do not pro duce oxygen during photosynthesis. The process of photosynthesis in the bacteria and in higher plants is discussed more fully below. The DeinococcusThermus are a small group of Gram negative bacteria comprised of cocci which are highly resistant to environmental hazards because they are able to quickly repair damage to their DNA. There are two main groups. The Deinococcales include a single genus, Deino coccus, with several species that are resistant to radiation; they have become famous for their ability to "eat" nuclear waste and other toxic materials, survive in the vacuum of atmosphere space, and survive extremes of heat and cold. Thermus spp. include several genera resistant to heat. Deino coccus radiodurans is an extremophilic bac terium, and is the most radioresistant organ ism known. It can survive heat, cold, dehydration, vacuum, and acid, and because of its resistance to more than one extreme condition, D. radiodurans is known as a polyextremophile. Thermus aquaticus is important in the develop ment of the polymerase chain reaction (PCR) where repeated cycles of heating DNA to near boiling make it advantageous to use a thermostable DNA polymerase enzyme. These bacteria have thick cell walls that give them Grampositive stains, but they include a second membrane and so are closer in structure to those of Gramnegative bacteria. Spirochetes are Gramnegative bacteria, which have long, helically coiled cells. Spirochetes are chemoheterotrophic in nature, with lengths between 5 and 250 mm and diameters around 0.1-0.6 mm. Spirochetes are distinguished from other bacterial phyla by the presence of flagella, sometimes called axial filaments, running length wise between the cell membrane and an outer membrane. These cause a twisting motion which allows the spirochete to move about. The spiro chete shape may also be described as consisting of an axial filament around which the cell is wound giving spirochetes their characteristic corkscrew shapes. Most spirochetes are freeliving and anaer obic, but they also include the following disease causing members: • Leptospira species, which causes leptospirosis (also known as Weil's disease) • Borrelia burgdorferi, which causes Lyme disease • Borrelia recurrentis, which causes relapsing fever • Treponema pallidum, which causes syphilis 7. Green sulfur bacteria Green Sulfur Bacteria are found in anaerobic environments such as muds, anaerobic, and sul fidecontaining fresh or marine waters, and wet lands. These anoxygenic phototrophic bacteria live in environments where light and reduced sulfur compounds are present. They are found most often under the Purple Sulfur bacterial layer. Green sulfur bacteria are capable of using sulfide or elemental S as the electron donor. The elemental S arises from H 2 S oxidation and is deposited extracellularly, before the oxidation of sulfate. There are four genera of green sulfur bacteria, Chlorobium, Prosthecohloris (with stalks or prostheca), Pelodictyon (with vacuoles), and Clathrochloris (motile). The Green Sulfur Bacteria strains are green because of the presence of bacteriochlorophylls (bchls) "c" and "d" and small traces of bchl "a" located in chlorobium vesicles attached to the cytoplasmic membrane. Some are brown and they contain bacteriochlorophyll "e." These brown strains are found in the deeper layers of wetlands and water. Both of the two groups can be found also living in extreme conditions of salinity and high temperatures. The morphology of both color types is most often either straight or curved rods. They are nonmotile phototrophic short to long rods which utilize H 2 S as electron donor oxidizing it to SO 2 and to SO 4 2+ . The sulfur so produced lies outside the cells. Light energy absorbed by Bacteriochlorophylls c, d, or e is channeled to Bacteriochlorophyll a, which actually carries out photosynthetic energy conversion, and ATP syn thesis takes place. A wellknown member is Chlorobium tepidum. In marine environments, they are found in the water column where hydrogen sulfide diffuses up from anaerobic sediments and where oxygen dif fuses down from surface waters where oxygenic photosynthesis is taking place. In the Black Sea, the largest anoxic water body in the world, they are found at a depth of 100 m (Manske et al. 2008) . They also live in special tissues in invertebrates such as Riftia pachyptila (vestimentiferan tube worms) and Calyptogena magnifica ("giant" white clams) that live around deep sea hydrothermal vents. There they provide energy, by oxidizing reduced sulfur compounds, and organic matter, by converting car bon dioxide to organic compounds, which the inver tebrates use. They are sometimes abundant in coastal waters, and several members of the group have gas vacuoles in their cells to help them float. Flavobacteria are Gram negative rods that are motile by gliding and found in aquatic environ ments, both freshwater and marine, and in the soil. Colonies are usually yellow to orange in color, hence their name. Flavobacteria are a group of commensal bacteria and opportunistic pathogens. Flavobacterium psychrophilum causes the septi cemic diseases of rainbow trout fry syndrome and bacterial cold water disease. They decompose sev eral polysaccharides including agar but not cellu lose. The type species is F. aquatile. These are thermophilic, anaerobic, chemolithoau totrophic Gram negative straight to bent rods. They can use a wide range of electron acceptors including Fe 3+ and Mn 2+ . They are found in a wide range of aquatic environments including deepsea hydrothermal vents. A wellknown member is Deferribacter desulfuricans 10. Cytophaga Cytophaga are unicellular, Gramnegative gliding bacteria. They are rodshaped, but specific strains differ in diameter and length with some being pleomorphic (many shaped). The type species is C. johnsonae, which has a moderately long thin shape. Many strains are red, yellow, or orange because of unique pigments synthesized by the group. Cytophaga strains tend to be versatile in making these and one strain may synthesize 25 different structural varieties of pigment. The main habitats of Cytophaga are soils at or close to neu tral pH, decaying plant material, and dung of ani mals. In freshwater environments, they are found on riverbanks and lake shores, in estuaries, bottom sediments, and algal mats. They are also common in sewage treatment plants, especially at the latter stages where only recalcitrant molecules remain. Cytophaga tend to degrade polymers such as cel lulose and have been shown to be the major cellu lose degraders in some lakes. A few species have been isolated from the oral cavity of humans where they appear to be part of the normal flora, but can occasionally cause septicemias. Some Cytophaga strains are pathogens of fish. 11. Planctomyces/Pirella Planctomyces, Pirella, Gemmata, and Isosphaera form a phylogenetically related group of microor ganisms that have many unusual properties. They are the only bacteria, other than the confusing case of the Chlamydia, whose cells lack peptidoglycan. Cells of this group divide by budding. Some mem bers of the group produce long appendages, called stalks, and new cells are motile, developing stalks as they mature. Some members of this group have structures resembling nuclear membranes (Bauld and Staley 1976) : others have fimbrin. Cells of this group can be pigmented (light rose, bright red, or yellow to ochre) or nonpigmented. An example of the species is Planctomyces limno philus, which is ovoid, has a diameter of 1.5 mm, and forms red pigmented colonies. It grows slowly at temperatures between 17°C and 39°C and takes at least a week to form colonies. Stalks of the organism are very thin and cannot be seen by light microscopy. These stalks appear to be made of thin fibers twisted into a bundle that emanates from one pole of the ovoid cell. Cells multiply by budding and new cells are motile and stalkless, but eventually grow stalks as part of a maturation process similar to that seen for Caulobacter. These microbes are common inhabitants of freshwater lakes, marine habitats, and salt ponds, but most have been difficult to isolate in pure culture. For example, three of the four species in Planctomyces have only been observed in lake water and never isolated. Verrucomicrobia, with the best example as Verrucomicrobia spinosum, has been isolated from freshwater, soil environments, and human feces. It produces cytoplasmic appendages called prosth eca. Prostheca are like warts and the name of the group comes from the Greek word for warts. Both mother and daughter contain prostheca at the time of the cell division. Chlamydia are obligate intracellular pathogens with poor metabolic capabilities. They cannot syn thesize biomolecules such as amino acids which they obtain from their hosts. Many Chlamydiae coexist in an asymptomatic state within specific hosts, and it is widely believed that these hosts pro vide a natural reservoir for these species. Chlamydiae exist in two states: a metabolically inert elementary body (EB) and a metabolically active reticulate body (RB) found only inside cells. EB is similar to the virions of viruses and enters the body by phagocytosis. Once ingested and inside the cell, EB divides and becomes RB. After it has killed the cell, it becomes EB again and is ready to be transmitted. Chlamydiae are spread by aerosol or by contact and require no alternate vector. Diseases caused by Chlymidia include sexually transmitted infections (STIs) (Chlamydia tracho matosis), pneumonia (Chlamydia pneumoniae), and bird pneumonia (Chlamydia psittaci). 14. Cyanobacteria Cyanobacteria (Greek: kuanόs (kyanós) = blue + bacterium) obtain their energy through photosyn thesis. They are often referred to as bluegreen algae, because they were once thought to be algae. They are a significant component of the marine nitrogen cycle system and an important primary producer in many areas of the ocean. Their ability to perform oxygenic (plantlike) photosynthesis is thought to have converted the reducing atmosphere of the early earth into an oxidizing one, which dra matically changed the life forms on Earth and provoked an explosion of biodiversity. Cyanobacteria are found in almost every conceivable habitat, from oceans to freshwater to bare rock to soil. Most are found in freshwater, while others are marine, occur in damp soil, or even tempo rarily moistened rocks in deserts. A few are endo symbionts in lichens, plants, various protists, or sponges and provide energy for the host. Some live in the fur of sloths, providing a form of camouflage. Cyanobacteria include unicellular and colonial species. Colonies may form filaments, sheets, or even hollow balls. Some filamentous colonies show the ability to differentiate into several differ ent cell types: vegetative cells, the normal, photo synthetic cells that are formed under favorable growing conditions; akinetes, the climateresistant spores that may form when environmental condi tions become harsh; and thickwalled heterocysts, which contain the enzyme nitrogenase, vital for nitrogen fixation. Heterocysts may also form under the appropriate environmental conditions (anoxic) wherever nitrogen is necessary. Heterocyst forming species are specialized for nitrogen fixa tion and are able to fix nitrogen gas, which cannot be used by plants, into ammonia (NH 3 ), nitrites (NO 2 − ), or nitrates (NO 3 − ), which can be absorbed by plants and converted to protein and nucleic acids. The rice paddies of Asia, which produce about 75% of the world's rice, do so because of the high populations of nitrogenfixing cyanobacteria in the rice paddy fields. Photosynthesis in cyanobacteria generally uses water as an electron donor and produces oxygen as a byproduct, though some may also use hydrogen sulfide as is the case among other photosynthetic bacteria. Carbon dioxide is reduced to form carbo hydrates via the Calvin cycle. In most forms, the photosynthetic machinery is embedded into folds of the cell membrane, similar to thylakoids found in the chloroplasts of higher plants. The cyanobacteria are traditionally classified by morphology into five sections, I-V: Chroo coc cales, Pleurocapsales, Oscillatoriales, Nostocales, and Stigonematales. The latter two contain hetrocysts. The members of Chroococcales are unicellular and usually aggregated in colonies. In Pleurocapsales, the cells have the ability to form internal spores (baeocytes). In Oscillatorialles, the cells are singly arranged and do not form special ized cells, (akinets and heterocysts). In Nostocalles and Stigonematalles, the cells have the ability to develop heterocysts under certain conditions. 15. Gram positive bacteria (including Mycoplasmas and Actinobacteria) Like the Proteobacteria, the Gram positive bacteria are very diverse; they contain many bacteria encoun tered in everyday life as agents of disease and inputs of production in industry or as important organisms in food microbiology. Some of them (the Mycoplasma) lack cell walls. Grampositive bacteria fall into two major phylo genetic divisions, "low-G + C" and "high-G + C.": (a) Low G + C group: G + C below 50%; (b) High G + C group: G + C higher than 50% (a) Low G + C Group: G + C Below 50% Nonsporulating Low G + C Group Staphylococcus: The staphylococci have spherical cells often found in groups resem bling clusters of grapes. Bacteria of this genus were originally grouped with other sphe rical microorganisms, especially of the genus Micrococcus, since these two genera often shared similar habitats. However, physiological studies and phylogenetic analysis have shown that these two genera are very different from one another. The differences between staphy lococci and micrococci are discussed below. Lactic Acid Bacteria: The lactic acid bacteria are Grampositive rods and cocci that produce lactic acid as their primary end product. An important group characteristic is the absence of cytochromes, porphyrins and respiratory enzymes. They are therefore incapable of oxi dative phosphorylation or any type of respira tion and are totally dependent on fermentation. Lactic acid bacteria do, however, contain mechanisms to deal with the toxic byproducts of oxygen, which categorizes them as aeroto lerant anaerobes. They include Streptococcus, Leuconostoc, Pediococcus, Lactococcus, Enterococcus, and Lactobacillus. Lactic acid bacteria are primarily differentiated based on the types of end products they form. Homo fermentative lactic acid bacteria produce only lactic acid as an end product, while heterofer mentative lactic acid bacteria produce lactate, ethanol, and CO 2 as well (Axelssson and Ahrne 2000; Narayanan et al. 2004 ). Bacillus: These are sporeforming aerobic rods. Bacillus is a genus of rodshaped, beta hemolytic Grampositive bacteria. Bacillus species are catalasepositive obligate or facul tative aerobes. Ubiquitous in nature, Bacillus includes both freeliving in soil, water and air, as well as some pathogenic species. Under stressful environmental conditions, the cells produce endospores resistant to heat, radiation, chemicals and other unfavorable conditions. Clostridium: These are Grampositive spore forming obligately anaerobic rods. Individual cells are rodshaped, and the name comes from the Greek for spindle. Clostridium includes common freeliving bacteria as well as important pathogens, including C. botuli num, an organism producing a very potent toxin in food; C. difficile, which can overgrow other bacteria in the gut during antibiotic ther apy; C. tetani, the causative organism of teta nus; C. perfringens, formerly called C. welchii, which causes a wide range of symptoms, from food poisoning to gas gangrene. Because C. perfringens produces much gas, it is also used as a replacement for yeasts in breadmak ing. C. sordellii has been linked to the deaths of more than a dozen women. They are impor tant in the anaerobic conditions of muds. Heliobacteria: Heliobacteria are strictly anaerobic, sporeforming photoheterotrophic members of the Firmicutes. 16s rRNA studies put them among the Firmicutes (Bacillus and Clostridium) but they do not stain Gram positively like the other members. They have no outer membrane and like certain other fir micutes (clostridia), they form heat resistant endospores. They are the only firmicutes known to conduct photosynthesis. Soluble periplasmic components appear absent in heliobacteria and photosynthesis takes place at the cell membrane, which does not form folds or compartments as it does in purple pho totrophic bacteria. A particularity of heliobac terial photosynthesis is the occurrence of a unique Bacteriochlorophll (BChl) g. BChl g is chemically closer to Chl a than to BChl a. Correspondingly, heliobacteria appear to be more closely related to oxygenic photosynthe sis than the green sulfur bacteria (based on 16SrRNA phylogeny as well as on trees built from sequences of the photosynthetic reaction center). A small group, it is the only known phototrophic one among the Gram positives. Heliobacteria consist of three genera, Heliobacterium (3 spp.), Heliobacillus (1 sp.), and Heliophilum (1 sp.). They cannot tolerate sulfide, all known species can fix nitrogen. They are common in the waterlogged soils of paddy fields. (b) High G + C Group: G + C Above 50% These include Actinomycetes, Mycobacteria, Micrococcus, and Corynebacterium: Actinomycetes Actinomycetes are filamentous and spore forming (non heat resistant spores), found in soil. They are very important as antibiotic pro ducers. Typical example is Streptomyces sp. They include some of the most common soil life, playing an important role in decomposi tion of organic materials, such as cellulose and chitin and thereby playing a vital part in organic matter turnover and carbon cycle. Actinomycetes of the family Actinoplanaceae, especially Actinoplanes, are readily isolated from the flowing waters of rivers and streams, where they are important in the decomposi tion of wood and other cellulolisic materials. This is a slowgrowing acidfast strain (Ziel-Nieelsen stain) implicated in diseases (M. lep rae, leprosy; M. tuberculosis, tuberculosis). Many are however freeliving and inhabit aquatic environments. These environmental or waterborne mycobacteria (WBM) inhabit a diverse range of natural environments and are a frequent cause of opportunistic infection in human beings and livestock. Several hospital and community outbreaks of mycobacterial infections, including infections as diverse as lifethreatening pneumonia in patients with arti ficial ventilation, cystic fibrosis, and chronic granulomatous disease; outbreaks of skin infec tion following liposuction; furunculosis after domestic footbaths; mastitis after body piercing; and abscess formation in intravenous drug users. Corynebacterium is a genus of Grampositive, facultatively anaerobic, nonmotile, rodshaped actinobacteria. Most do not cause disease, but are part of normal human skin flora. Coryne bacterium diphtheriae is the cause of diphtheria in humans. The genes encoding exotoxins that are the cause of diphtheria (caused by Corynebacterium) as well as cholera and some other bacterial diseases are mobile in aquatic and terrestrial environments and have been found in sediments and in river water using PCR. These are cocci in bunches and very similar to staphylococci. They are distinguished from each other according to the properties shown in Table 4 .7. Nitrospira are nitriteoxidizing bacteria that are important in marine habitats. In aquaria, for exam ple, if the ammonia/nitrite/nitrate cycle is exhausted, the ecosystem suffers and fish can get sick or die. Therefore, nitriteoxidizing bacteria as well as the other bacteria in this system are important for healthy marine ecosystems. In addition, Nitrospira like bacteria are the main nitrite oxidizers in waste water treatment plants. The Proteobacteria are a major group of bacteria. They include a wide variety of pathogens, such as Escherichia, Salmonella, Vibrio, and Helicobacter. Others are important agriculturally or industrally; still others are freeliving, and include many of the bacteria responsible for nitrogen fixation. The group is defined primarily in terms of ribosomal RNA (rRNA) sequences, and is named after the Greek god Proteus, who could change his shape, because of the great diversity of forms found within the group. Proteus is also the name of a bacterial genus within the Proteobacteria. All Proteobacteria are Gramnegative, with an outer membrane mainly composed of lipopolysac charides. Many move with flagella, but some are nonmotile or move by bacterial gliding. The latter include the myxobacteria, a unique group of bac teria that can aggregate to form multicellular fruit ing bodies. There is also a wide variety in the types of meta bolism. Most members are facultatively or obligately anaerobic and heterotrophic, but there are numerous exceptions. A variety of genera, which are not closely related to each other, convert energy from light through photosynthesis. These are called purple bacteria, referring to their mostly reddish pigmentation. The Proteobacteria are divided into five sec tions, referred to by the Greek letters alpha through epsilon, again based on rRNA sequences. The Alphaproteobacteria comprise the most pho totrophic genera, but also several genera meta bo lizing C1compounds (compounds with a single carbon atom e.g., Methylobacterium, symbionts of plants (e.g., Rhizobia) and animals, and a group of intracellular pathogens, the Rickettsiaceae. Moreover, the precursors of the mitochondria of eukaryotic cells are thought to have originated in this bacterial group. The Betaproteobacteria consist of several groups of aerobic or facultative bacteria which are often highly versatile in their degradation capacities, but also contain chemolithotrophic genera (e.g., the ammoniaoxidizing genus Nitrosomonas) and some phototrophs (genera Rhodocyclus and Rubrivivax). Beta Proteobacteria play an important role in nitro gen fixation in various types of plants, oxidizing ammonium to produce nitrite an important chemi cal for plant function. Many of them are found in environmental samples, such as waste water or soil. Pathogenic species within this class are the Neisseriaceae (gonorrhea and meningoencephali tis) and species of the genus Burkholderia. The Gammaproteobacteria comprise several medically and scientifically important groups of bacteria, such as the Enterobacteriaceae, Vibrion aceae, and Pseudomonadaceae. Many important pathogens belong to this class, e.g., Salmonella (enteritis and typhoid fever), Yersinia (plague), Vibrio (cholera), Pseudomonas aeruginosa (lung infections in hospitalized or cystic fibrosis patients), and E coli. The Deltaproteobacteria comprise a group of pre dominantly aerobic genera, the fruiting body forming myxobacteria, and a branch of strictly anaerobic genera, which contains most of the known sulfatereducing bactria, (Desulfovibrio, Desulfobacter, Desulfococcus, Desulfonema, etc.) and sulfurreducing bacteria (e.g., Desulfuromonas) alongside several other anaerobic bacteria with different physiology (e.g., ferric ironreducing Geobacter and Pelobacter and Syntrophus species, which live symbiotically together). The Epsilonproteobacteria consist of only a few genera, mainly the curved to spiralshaped Wolinella, Helicobacter, and Campylobacter. Most of the known species inhabit the digestive tract of animals and humans and serve as symbi onts (Wolinella in cows) or pathogens (Helicobacter in the stomach and Campylobacter in the duode num in humans). There have also been numerous environmental sequences of epsilons recovered from hydrothermal vent and cold seep habitats. This section will discuss the physiology of some of the activities of aquatic microorganisms which con tribute to their ecology in bodies of water as well as to their economic importance. Items to be discussed are photosynthesis, nitrogen economy, especially nitrogen fixation, sulfate reduction, and iron in the aquatic environment. Photosynthesis is the conversion of CO 2 to carbohy drates using light energy. This process has been described as the most important biological reaction on earth, since it is the means by which the energy of the sun is harnessed by living things, through their consumption of the products of photosynthesis. Photo synthesis is carried out by plants, algae, and some bacteria, but not by Archae. It is an important factor affecting the ecol ogy of microorganisms in aquatic environments (Achenbach et al. 2001) . Photosynthesis is generally better known in plants than in bacteria; plant photosyn thesis will therefore be discussed as a basis for under standing bacterial photosynthesis (see Fig. 4 .11). Photosynthesis is hinged on three items: (a) Photosynthetic pigments, (b) the light or lightdepen dent reactions of photosynthesis, and (c) the dark or lightindependent reactions of photosynthesis. A pigment is any substance that absorbs light. The color of the pigment comes from the wavelengths of light reflected by the pigment (in other words, those not absorbed). Chlorophyll, the green pigment com mon to all photosynthetic cells, absorbs all wave lengths of visible light except green, which it reflects, and thus is detected by human eyes as green. Black pigments absorb all of the wavelengths that strike them. White pigments/lighter colors reflect all or almost all of the light energy striking them. Pigments have their own characteristic absorption spectra, the absorption pattern of a given pigment. Chlorophyll (chl) found in plants, algae, and cyanobacteria, is very similar to bacteriochlorophyll (bchl) found in bacteria, other than cyanobacteria (see Fig. 4 .12). There are several types of chlorophylls and of bacteriochlorophylls, (named a, b, c, d, e, and g) differing from each in slight differences in structure. Bchls "a" and "b" are found in the purple bacteria; while bchls "c," "d," and "e" are found in Green sulfur bacteria; bchl "g" is found in Heliobacteria. In higher plants, photosynthesis takes place only in chl "a"; all other chlorophylls along with carotenoids are acces sories and gather light which is channeled to chl "a." Similarly, in bacteria, bchl "a" is the site of photosyn thesis; all the other bacteriochlorophylls are accesso ries and gather light which is channeled to bchl "a." Accessory pigments include carotenoids found in higher plants and cyanobacteria and phycobilins found in the algae. Pigments have their own characteristic absorption spectra. Figure 4 .13 shows the wavelength of various chlorophylls and accessory pigments. In higher plants, the light dependent reactions, take place on membranous structures known as thylakoids found in chloroplasts in complex processes, that are not yet fully understood. The process is much simpli fied as described below. In plants, light is absorbed by complexes formed between protein and chlorophyll molecules known as photosystems, Photosystem I (PSI) and Photosystem II (PSII). PSII absorbs light energy (photons) at a wave length of 680 nm and is called P680 while PSI it absorbs photons at 700 nm and is called P700. When a pigment absorbs light energy, one of three things will occur: Energy may be dissipated as heat; it may be reemitted immediately as a longer wavelength, a phenomenon known as fluorescence; or the energy may trigger a chemical reaction, as in photosynthesis. In plant photosynthesis, the action begins at the PSII chlorophyll-protein complex which becomes excited and loses an electron; this electron is passed through a series of enzymes until it is transferred to water, causing it to lose electrons: The electron released from the splitting of water is transferred to PSI, which can itself capture light energy; this energy is transferred by enzymes used to reduce NADP + to NADPH and ATP the other energy currency of cells, thus ADP + Pi ⇒ ATP. While the photosynthetic process in cyanobacteria is similar to that of plants, green bacteria and purple sulfur bacteria have photosynthetic processes different from the process in plants. Cyanobacteria do not have chloroplasts, but have structures on their cell membranes which are similar to thylakoids. They have photosystems similar to PS II and PS I found in the chloroplasts of higher plants. They can produce NADPH and ATP in the way as higher plants and they are the only bacteria which produce O 2 during photosynthesis. However, instead of carotenoids or chlorophyll "b" which act as accessory pigments in higher plants, they have phycobilins. Purple Bacteria: Purple bacteria and green sulfur bacteria have only one type of photosystem. The single photosystem in purple bacteria is structurally related to PS II in cyanobacteria and plant chloroplasts; it, however, has a P870 molecule, i.e., it absorbs light at 870 nm and can make ATP in the transfer of electrons. In order to make NADPH, purple bacteria use an external electron donor (hydrogen, hydrogen sulfide, sulfur, sulfite, or organic molecules such as succinate and lactate) to feed electrons into a reverse electron transport chain. Green Sulfur Bacteria: These bacteria contain a pho tosystem that is analogous to PS I (P840) in chloro plasts. It makes ATP through the transfer of electrons. Electrons are removed from an excited chlorophyll molecule and used to reduce NAD + to NADH. The electrons removed from P840 must be replaced. This is accomplished by removing electrons from H 2 S, which is oxidized to sulfur which appear as globules in the cells (hence the name "green sulfur bacteria"). for the production of energy rich carbohydrates ( sugars) in the Calvin cycle (see Fig. 4 .11). The fixation or reduction of carbon dioxide is a lightindependent process in which carbon dioxide combines with a fivecarbon sugar, ribulose 1,5bis phosphate (RuBP), to yield two molecules of a three carbon compound, glycerate 3phosphate (GP), also known as 3phosphoglycerate (PGA). GP, in the pres ence of ATP and NADPH from the lightdependent stages, is reduced to glyceraldehyde 3phosphate (G3P) and enters the citric acid cycle. The processes of photosynthesis can be represented by the general formula: where H 2 A is the source of the reducing power for the conversion of CO 2 to carbohydrates. In higher plants, algae and cyanobacteria, where water is the source of the reducing power photosynthe sis, can be represented thus: In bacteria, other than cyanobacteria, where water is not the source of reducing power and hence oxygen is not involved (anoxygenic), for example, the green sulfur bacteria, where hydrogen sulfide is utilized, the photosynthetic equation is given thus: Like green plants, some bacteria are photosynthetic, using the energy of sunlight to reduce carbon dioxide to carbohydrate. There are a number of differences between the two groups which are summarized below: Chlorophyll, the photosynthetic pigment in plants, is replaced in bacteria by bacteriochlorophyll (except in the Cyanobacteria). Both types of pigments are similar and differ only in some side chains (see Fig. 4 .12). In higher plants, photosynthesis takes places in membraneous structures known as thylakoids which are located in organelles known as chloroplasts. In bacteria, the site for photosynthesis varies from one group of bacteria to the other. In the cyanobacteria, although chloroplasts are absent, photosynthesis occurs in thylakoidlike structures; in helicobacte ria, it takes place on the cell membranes; in the purple bacteria, it takes place in invaginations of the cell membrane; in the green bacteria, it takes place on the cell membrane as well as in special membrane folding known as chlorosomes. In higher plants, algae and cyanobacteria, the light energy excites the molecules of chlorophyll leading to release of energy which splits the water molecule and to the release of oxygen as a byproduct, and finally the provision of H for fixing the CO 2 . In most bacteria (apart from cyanobacteria), oxygen is not released because water does not provide the H which converts the CO 2 to carbohydrates. Rather, light energy excites bacteriochlorophyll leading to energy which splits H from H 2 S. In the dark, many photosynthetic bacteria can produce energy by the transfer of electron, or anaerobically. The photosynthetic bacteria can be divided into two groups: The anaerobic photosynthetic groups and the aerobic photosynthetic bacteria. The bacterial order Rhodospirillales contains three photosynthetic families: (a) Rhodospirillaceae: Purple nonsulfur bacteria, e.g., Rhodospirillum. These cells contain bacte riochlorophyll "a" or "b" located on specialized membranes continuous with the cytoplasmic membrane. They are not able to use elemental sulfur as electron donor and typically use an organic electron donor, such as succinate or malate, but can also use hydrogen gas. (b) Chromatiaceae: These include purple sulfur bac teria, e.g., Chromatium. They are able to use sul fur and sulfide as the sole photosynthetic electron donor and sulfur can be oxidized to sulfate. They can use inorganic sulfur compounds, such as hydrogen sulfide as an electron donor. Purple sul fur bacteria must fix CO 2 to survive, whereas non sulfur purple bacteria can grow aerobically in the dark by respiration on an organic carbon source. They store elemental sulfur inside their cells, and these appear globules within their cells, hence their name, purple sulfur bacteria. (c) Chlorobiaceae: These are green sulfur bacteria; their cells contain bacteriochlorophyll "c" or "d" located in chlorobium vesicles attached to the cytoplasmic membrane. (d) Heliobacteria: The heliobacteria are anaerobic and phototrophic, converting light energy into chemical energy by photosynthesis using a PSI type reaction center (RC) (P798). The primary pigment involved is bacteriochlorophyll g, which is unique to the group and has a unique absorp tion spectrum. On account of this, the heliobac teria occupy their own special environmental niche. Phototrophy takes place on the cell mem brane, which does not form folds or compart ments as it does in purple phototrophic bacteria. Using 16 S RNA analysis, they are placed among the Firmicutes, Gram positive bacteria; although, they do not stain Gram positive, but they form heat resistant endospores. Heliobacteria are the only fir micutes known to conduct photosynthesis. They are photoheterotrophic, i.e., they require organic car bon sources. They do not fix carbon dioxide, they lack rubisco, and do not have Calvin cycle. They are found in soils, especially water logged soils such as in paddy fields. They are also strong nitrogen fixers. The cyanobacteria are photosynthetic and aerobic, but recently another photosynthetic aerobic group was discovered. It was previously generally believed that anoxygenic photosynthesis was an anaerobic growth mode of either obligately anaerobic, or fac ultatively anaerobic bacteria capable of switching between respiration under aerobic conditions and phototrophy under anaerobic conditions. Recently (1979), the first reported member of the aerobic phototrophic bacteria, Erythrobacter longus, discovered in the Bay of Japan, changed our previous knowledge of the phototrophic bacteria. APBs have since been found in a wide variety of both marine and freshwater habitats, including acid mine drainage sites, soils, saline lakes, and soda lakes. (Rathgeber et al. 2004) . Other genera of APBs found in freshwater and marine envi ronments include the following: Erythrobacter,, Roseobacter,, Porphyro bacter,, Acidiphilium Erythromonas, Erythromi crobium, Roseococcus, and Sandaracinobacter. The APBs produce a photosynthetic apparatus similar to that of purple phototrophic bacteria. However, this apparatus, in contrast to that of the anaerobic photosynthetic bacteria is produced only under aerobic conditions. In facultatively anaero bic organisms, the photosynthetic apparatus is syn thesized under conditions of oxygen shortage and absence of light. They are a phylogenetically diverse group inter spersed predominantly throughout the aProteobac teria, closely related to anoxygenic phototrophic purple nonsulfur bacteria as well as chemotrophic species. Recently, however, more and more APBs have been placed in the bProteobacteria. Nitrogen is important in microorganisms for the manu facture of proteins and nucleic acids, both of which are essential for the continued existence of all living things. Although the element is abundant in the atmosphere, constituting about 80%, the ability of making atmo spheric nitrogen available to living things is present only in a few organisms. Biological nitrogen fixation can be represented by the following equation, in which 2 moles of ammonia are produced from 1 mole of nitrogen gas, at the expense of 16 moles of ATP and a supply of electrons and protons (hydrogen ions): This reaction is performed exclusively by prokaryotes using a nitrogenase enzyme complex. This enzyme consists of two proteins -an iron protein and a molybdenumiron protein -as shown Fig. 4 .14. The reactions occur while N 2 is bound to the nitroge nase enzyme complex. The Fe protein is first reduced by electrons donated by ferredoxin. Then the reduced Fe pro tein binds ATP and reduces the molybdenum-iron protein, which donates electrons to N 2 , producing HN=NH. In two further cycles of this process (each requiring electrons donated by ferredoxin), HN=NH is reduced to H 2 N-NH 2 , and this in turn is reduced to 2NH 3 . Depending on the type of microorganism, the reduced ferredoxin, which supplies electrons for this process, is generated by photosynthesis, respiration, or fermentation (Anonymous 2010e) . Nitrogen fixation may be done by bacteria living symbiotically with higher plants such as Rhizobium spp. and legumes or by freeliving organisms. In the aquatic environment, the nitrogen fixers are freeliving microorganisms including aerobic and anaerobic ones. (Naqvi 2006) . Among aerobes, nitrogen fixers include all members of Azotobacter and Beijerinckia,, some Klebsiella and some cyanobacteria. Under anaerobic conditions, such as, occur in sediments or in the deeper regions of water columns, the following organisms fix nitrogen: Some Clostridium spp., Desulfovibrio, pur ple sulfur bacteria, purple nonsulfur bacteria, and green sulfur bacteria. The nitrogenase enzyme complex is highly sensitive to oxygen and it is inactivated when exposed to oxy gen, because oxygen reacts with the iron component of the proteins. Aerobic organisms including cyanobac teria, which produce oxygen during photosynthesis, combat the problem of nitrogenase inactivation by different methods. Cyanobacteria for example have special cells, heterocysts, where nitrogen fixation occurs and in which nitrogenase is protected because they contain only photosystem I whereas the other cells have both photosystem I and photosystem II (which generates oxygen when light energy is used to split water to supply H 2 in photosynthesis.). For the same reason, also, Azotobacter and Rhizobium pro duce large amounts of extracellular polysaccharide, which helps limit the diffusion of oxygen to the cells. Furthermore, Rhizobium root nodules contain oxygen scavenging molecules such as leghemoglobin, which regulate the supply of oxygen to the nodule tissues in the same way as hemoglobin regulates the supply of oxygen to mammalian tissues. Other microbial activities which participate in regulating the nitrogen economy of aquatic systems are nitrification and denitrification. Nitrification is the conversion of ammonium to nitrate by the nitrifying bacteria. These bacteria are chemo autothrophs which obtain energy by oxidizing ammo nium, while using CO 2 as their source of carbon to synthesize organic compounds. The nitrifying bacteria are found in most soils and waters of moderate pH, but are not active in highly acidic soils. They almost always are found as mixedspecies communities or consortia. Some of them -e.g., Nitrosomonas convert ammonium to nitrite (NO 2 − ) while others -e.g., Nitrobacter convert nitrite to nitrate (NO 3 − ). The nitrifying bacteria are so numerous in waters rich in ammonium such as sewage effluents that they readily convert the ammonium compounds therein into nitrates. The nitrates can accu mulate in groundwater, and may ultimately enter drinking water. Regulations in many countries control the amount of nitrate in drinking water, because in the anaerobic conditions of the animal alimentary canal, nitrates can be reduced to highly reactive nitrites by microorganisms. Nitrites are absorbed from the gut and bind to hemoglobin, reducing its oxygencarrying capacity. In young babies, this can lead to a respiratory illness known as blue baby syndrome. Nitrites can also react with amino compounds, forming nitrosamines which are highly carcinogenic. Denitrification is the conversion of nitrate to gaseous compounds (nitric oxide, nitrous oxide, and N 2 ) by microorganisms. Denitrification goes through some combination of the following intermediate forms: The denitrification process can be expressed in terms of electron transfer thus: Denitrification is brought by a large number of different bacteria which are mainly heterotrophic. They complete the nitrogen cycle by returning N 2 to the atmosphere. Denitrification occurs under special conditions in both soil and aquatic conditions, includ ing marine environments. Denitrification occurs when oxygen supply is low such as in ground water, wet lands in seafloors, and other poorly aerated parts of aquatic systems. The conditions which encourage den itrification are those in which there is a supply of oxi dizable organic matter, and absence of oxygen and the availability of reducible nitrogen sources. Under such conditions, the terminal electron acceptor for the deni trifying bacteria is not oxygen but the nitrogen com pounds given in the formula above. The organisms prefer nitrates and the other compounds in the equa tion, in the order they occur in the equation above and ending with nitrous oxide. When the terminal electron acceptor is an inorganic compound such as those in the formula above, the condition is also termed respiration as is also the case with oxygen. A mixture of gaseous nitrogen products is often produced because of the stepwise use of nitrate, nitrite, nitric oxide, and nitrous oxide as electron acceptors in anaerobic respiration. The commonest denitrifying bacteria include several species of Pseudomonas, Alkaligenes, Bacillus,, and Paracoccus denitrificans. Autotrophic denitrifiers (e.g., Thiobacillus denitrifi cans) have also been identified. In general, however, several species of bacteria are involved in the com plete reduction of nitrate to molecular nitrogen, and more than one enzymatic pathway have also been identified. In some organisms, direct reduction from nitrate to ammonium (also known as dissimilatory nitrate reduction to ammonium or DNRA) may also occur; although, this is less common than denitrification. Anammox, an abbreviation for ANaerobic AMMonium OXidation, is a globally important microbial process of the nitrogen cycle. It takes place in many natural environments. The bacteria mediating this process were identified only 20 years ago. They belong to the bacterial phylum Planctomycetes, of which Planctomyces and Pirellula are the best known genera. Four genera of anammox bacteria have been identified: Brocadia, Kuenenia, Anammoxoglobus, Jettenia (all freshwater species), and Scalindua (marine species). Note: Ferrodoxins are a group of redbrown proteins contain ing iron and sulfur, which act as electron carriers during photo synthesis, nitrogen fixation, or oxidationreduction reactions in green plants, algae, and anaerobic bacteria. Nitrogenase is a twoprotein complex. One component, nitrogenase reductase is an ironcontaining protein that accepts electrons from ferredoxin, a strong reductant, and then delivers them to the other component, nitrogenase, which contains Iron (Fe) and molybdenum (Mo). The overall reaction in nitrogen fixation via nitrogenase is: The anammox bacteria are characterized by several striking properties: (a) They all possess one anammoxosome, a membrane bound compartment inside the cytoplasm which is the site of anammox catabolism. (b) Further, the membranes of these bacteria mainly consist of ladderane lipids which are rare in living organisms. (c) Hydrazine (normally used as a highenergy rocket fuel, and poisonous to most living organisms) is a byproduct of these organisms. (d) Finally, the organisms grow very slowly, the gen eration or doubling time being nearly 2 weeks. The anammox process was originally found to occur only from 20°C to 43°C, but more recently, ana mmox has been observed at temperatures from 36°C to 52°C in hot springs and 60°C to 85°C at hydrothermal vents located in the ocean floor. Reduction under anaerobic conditions can also occur through anaerobic ammonia oxidation (Anammox) thus: Because denitrifying bacteria are principally het erotrophic, in some wastewater treatment plants, small amounts of methanol are added to the wastewater to provide a carbon source for the bacteria. Nitrogen fixation, nitrification, and denitrification are interlinked in the nitrogen cycle. The nitrogen cycle in the marine environment is given in Fig. 4.15 . In the environment, through changes brought about mostly by bacteria, sulfur changes from one form to the other: From hydrogen sulfide (H 2 S) to sulfate via elemental sulfur (S 0 ) and sulfate is changed again to hydrogen sulfide. Hydrogen sulfide is also evolved from hot springs and volcanoes, and occurs when dead animals, the excreta of animals, and dead plants are decomposed by bacteria. The compound is oxidized to sulfuric acid by the sulfuroxidizing bacteria and pho tosynthetic sulfur bacteria via elemental sulfur. The change of hydrogen sulfide to elemental sulfur occurs also abiotically in the presence of molecular oxygen. Dimethyl sulfide (CH 3 ) 2 S is produced by marine algae and marine cyanobacteria and contributes to the typical smell of thee sea. Dimethyl sulfide is degraded by bacteria such as Thiobacillus and Hyphomicrobium, leading to the formation of acid. The various transfor mations are summarized in Fig. 4.16 . A major group of bacteria important in the global economy of sulfur, especially in aquatic environments are the sulfate reduc ing bacteria. They will be discussed briefly below. The sulfate reducing bacteria (SRB) are ubiquitous anaerobes found in diverse environments. They include several groups of bacteria that use sulfate as an oxidiz ing agent, reducing it to sulfide (Fig 4.17) (Luptakova 2007) . They can also utilize other sulfur compounds, including sulfite, thiosulfate, and elemental sulfur in a type of metabolism known as dissimilatory, because sulfur is not converted into organic compounds. The rotten egg odor of hydrogen sulfide in the environment usually indicates the presence of sulfatereducing bac teria in nature. Sulfatereducing bacteria are responsi ble for the rotten egg odors of salt marshes, mud flats, and intestinal gas. They slowly degrade materials that are rich in cellulose in anaerobic environments. Apart from soil, sulfate reducing bacteria are found in various habitats such as seas and oceans, mud and sediments of freshwaters (rivers, lakes), waters rich in decaying organic material, thermal or nonthermal sulfur springs, mining waters from sulfide deposits, waters from deposits of mineral oil and natural gas, industrial waste waters from metallurgical industry, as well as in the gastrointestinal tract of man and animals (Barton and Hamilton 2007) . Based on the energy source of sulfate reducing bacteria, there are two types of anaerobic respiration of sulfates: autotrophic and heterotrophic. 1. Autotrophic reduction of sulfates: In this case, the energy source is gaseous hydrogen; the reaction proceeds in several stages and the whole process can be expressed by: During anaerobic respiration of sulfates, SRBs pro duce large amounts of gaseous hydrogen sulfide (H 2 S) which react easily in the water medium with heavy metal cations forming fairly insoluble metallic sulfides (Eq. 4.4): (4.4) SRBs are of great economic importance espe cially in the oil industry. They are ubiquitous in oil bearing shale and strata and therefore play an important economic role in many aspects of oil tech nology. They are: 1. Responsible for extensive corrosion of drilling and pumping machinery and storage tanks 2. Contaminate resulting crude oil and thereby increase undesirably the sulfur content of the oil through the H 2 S which they release into it 3. Important in secondary oil recovery processes, where bacterial growth in injection waters can plug machinery used in these processes 4. Speculated to play a role in biogenesis of oil hydrocarbons For all of these reasons, SRB are of vital importance in petroleum producing and processing industries. Apart from the above, SRB are responsible for the corrosion of buried tanks and tanks made of iron; in some industries, such as the paper industry, they cause undesirable blackening of paper due to iron sulfides in the processing water. In nature, sulfur circulates permanently because it is continuously oxidized or reduced by chemical or biological processes. In such a biogeochemical sulfur cycle (Fig. 4.16) , the biological transformations may have either assimilatory or dissimilatory metabolic functions. SRB play an important in this cycle. Figure 4 .16 shows the global sulfur cycle, including biological and nonbiological activities. The biological component of sulfur transformation is given in Fig. 4 .17. Most plants, fungi, and bacteria are capable of performing an assimilatory reduction of sulfate to sulfide which is necessary for the biosynthesis of sulfur containing cell compounds. On the other hand, the energy producing dissimilatory sulfur metabolism is restricted to a few groups of bacteria. The bacteria which participate in the dissimilatory section of the biological sulfur cycle are collectively known as the sulfuretum. These groups include: (a) Anaerobic dissimilatory sulfate reducers (Desul fovibrio, Desulfotomaculum, Desulfomonas) (b) Anaerobic dissimilatory sulfur reducers (Desul furomonas, Beggiatoa) (c) Anaerobic phototrophic sulfur oxidisers (some cyanobacteria and most anoxygenic phototrophic bacteria) (d) Anaerobic chemotrophic sulfur oxidisers (Thio bacillus denitrificans, Thiomicrospira denitrificans) Iron bacteria are chemoautotrophs which derive energy by oxidizing dissolved ferrous iron, and sometimes manganese and aluminum. The resulting ferric oxide is insoluble, and appears as brown gelatinous slime that will stain plumbing fixtures, and clothing or utensils washed with the water carrying the oxide. Iron bacteria grow in waters containing as low as 0.1 mg/l of iron. They produce the brownish scale that forms inside the tanks of flush toilets. They complete the oxidation of partially oxidized iron compounds and are able to couple the energy produced to the synthesis of carbohydrate. Many different bacteria can be involved in producing oxidized iron seen as "rusty" sediments in water. The true iron bacteria are those whose metabolism has been described above. The genera involved are Leptothrix,, Clonothrix, and Gallionella and Sphaerotilus.They are usually stalked, filamentous, and difficult or impossible to cultivate. They are sheathed and the outer portion of the sheaths is covered with slime in which oxides of iron are deposited giving them the colors ranging from red to brown. This sheath makes them somewhat resistant to disinfectants. Typical symptoms of iron bacterial growths in water supplies are: (a) Discoloration of the waters (yellow to rustred or brown) (b) Reduction in flow rates through the system caused by coatings of iron bacteria inside the pipes (c) Development of thick red or brown coatings on the sides of reservoirs, tanks, and cisterns; sometimes, sloughing off to form either fluffy specks in the water or gelatinous clumps of red to brown filamentous growths (d) Rapid Clogging of Filter screens (e) Heavy surface and sedimented growths of a red or brown color sometimes iridescent (ochre) in water Iron bacteria do not cause disease and their nuisance value is mainly esthetic. They cause economic loss due to stained porcelain fixtures, fouled laundry, etc. Iron bacteria are not active at temperatures of about 5°C or lower and they require water with iron content of at least 0.2 mg/l. They thrive in situations where there is good aeration, some source of nutrition, and some heat such as provided by water pumps, and a regular supply of water with dissolved iron. They are susceptible to ultraviolet of the sun and hence are found deep in the ground or hidden in pipes. Heavy growths of iron bacteria form a substrate for other bacteria which may then degrade these materials anaerobically to form acidic products and hydrogen sulfide. The growth of iron bacteria can controlled through the use of chlorine. It should be pointed out that passing that "rust" is not always solely due to bacterial activity but could be due to physicochemical reactions, especially where the geological formations contain iron oxides in the form of different iron minerals: Siderite (iron carbon ate), pyrite or greigite (iron sulfide) and hematite (iron oxide or hydroxide). Ground water is low in oxygen and has pH near neutrality. The dissolved iron oxides can rise to as high as 5 mg/l under these conditions. When the water is pumped from underground, it is exposed to air and the dissolved oxides are quickly oxidized and sediment as fine rusty colored powder. Oxidizing agents such as chlorine and potassium per manganate accelerate the oxidation of the oxides and deposition of rust. During water purification, the aeration of the raw also hastens the deposition of the oxides. Manganese oxides are frequently common in waters with iron oxides. They form black deposit when oxidized. Like the Domain Bacteria, the Domain Archaea consist of singlecelled organisms lacking nuclear membranes, and are therefore prokaryotes. A single organism from this domain is called an archaeon, just as a single member in the Domain Bacteria is a bacterium. As seen in Table 4 .1 the properties of Archaea make them closer, evolution arily, to Eukaryotes than they are to Bacteria. Thus their genetic transcription and translation do not show many typical bacterial features, and are in many aspects similar to those of eukaryotes. Many archaeal tRNA and rRNA genes harbor unique archaeal introns which are neither like eukaryotic introns, nor like bacterial introns. Several other characteristics also set the Archaea apart. Archaea lack a peptidoglycan wall. Even in this case, the peptidoglycan is very different from the type found in bacteria. Archaea are divided into two main groups based on rRNA trees, the. Two other groups have recently been tentatively added: Koracheota and Nanoarheota. The discussion will be on the first two, and better known, groups. Members of this group can be arranged as follows: 1. Extremely halohilic Archaea: Members of this group survive in hypersaline environments, high levels of salt, such as are found in Great Salt Lake in Utah, and the Dead Sea. All are known as extremely Halophilic Archaea stain Gram negative. There are ten genera and 20 species of extreme halophiles, five of these genera contain only one species each: Halobacterium; Halobaculum; Natrosobacterium; Natrialba; Natrosomonas. The other genera are: Natrarococcus (two species); Haloarcula (two species); Halococcus (two species); Haloferax (four species); Halorubrum (five species). The key genera in this group are Halobacterium,, Haloferax, and Natronobacterium. 2. Methane producing Archaea: Nearly half of the known species of Archaea are unique in being capa ble of producing methane energy from selected low molecular weight carbon compounds and hydrogen as part of their normal biochemical pathways. Methanogens are anaerobic and are the most com mon and widely dispersed of the Archaea being found in anoxic sediments and swamps, lakes, marshes, paddy fields, landfills, hydrothermal vents, and sewage works as well as in the rumen of cattle, sheep, and camels, the cecae of horses and rabbits, the large intestine of dogs and humans, and in the hindgut of insects such as termites and cockroaches. In their natural habitats, methanogens depend on substrate supply from associated anaerobic microbial communities or geological sources, and depending on the substrates they utilize, three types of methano genic pathways are recognized (see Fig. 4.18) : (a) Hydrogenotrophic methanogens which grow with hydrogen (H 2 ) as the electron donor and carbon dioxide (CO 2 ) as the electron acceptor. Some hydrogenotrophs also use formate, which is the source of both CO 2 and H 2 . (b) Acetoclastic methanogens which cleave acetate into a methyl and a carbonyl group. Oxidation of the carbonyl group into CO 2 provides potential for reduction of the methyl group into CH 4 . (c) Methylotrophic methanogens grow on methy lated compounds such as methanol, methy lamines, and methyl sulfides, which act as both electron donor and acceptor or are reduced with H 2 . The important genera among methane producing Archaea are Methanobacterium, Methanosarcina and Methanocaldococcus. Methanogens utilize a wide variety of substrates for producing methane. These include CO 2 , alcohols, methyl substrates, methanol (CH 3 OH), methylamine (CH 3 NH 3+ ), and trimethylamine ((CH 3 ) 3 NH + ) and acetic compounds such as acetate (CH 3 COO − ) and pyruvate. 3. Thermophilic and Extremely Acidophilic (Thermo plasmatales): This is a small group of extreme aci dophilic organisms. They containing four species in two genera, they are unusual in their ability to toler ate acid conditions. The two Picrophilus species are the most acidophilic organisms known. They have an optimal pH requirement of 0.7, can still grow at a pH of −0.06 and die at pH values of less than 4.0. Both Picrophilus species were found in acid solfa toras in Japan. Solfatoras are craters, often near vol canoes, spewing out steam, and gases such as CO 2 , SO 2 , and HCl. When sulfurous gases are spewed out from such craters they are solfatoras (from the Italian for sulfur). The two species of Thermoplasma grow optimally at pH 2.0. Thermoplasma spp. are also very unusual in that they do not have a cell wall. T. volcanium has been isolated from a number of solfatoras around the world. The cell membrane of Thermoplasma is composed of a lipopolysaccha ridelike compound consisting of lipid with man nose and glucose units and called a lipoglycan. Examples of this group are Thermoplasma and Ferroplasma. These Archae lack cellwalls and in this regard are like Mycoplasmas. They not only survive without cellwalls but they also survive high temperatures and low acid conditions. For these conditions, these organisms have special polysaccaride structures in their cell membranes, a lipopolyssacharide. 4. Hyperthermophilic Archae: Well-known members of this group are Thermococcus, Pyrococcus, and Methanopyrus. Members of this group have optimal temperatures of 80°C and many grow at tempera tures higher than that of boiling water. Thus Thermococcus and Pyrococcus (cocci with a tuft of flagella on one side) grow at between 70°c and 106°C with an optimum at 100°C (Pyrococcus). Proteins, starch or maltose are oxidized as electron donors and S 0 is the terminal acceptor and is reduced to H 2 S. Crenarchaeota has the distinction of including microbial species with the highest known growth temperatures of any organisms. As a rule, they grow best between 80°C and 100°C and several species will not grow below 80°C. Several species also prefer to live under very acidic conditions in dilute solutions of hot sulfuric acid. Approximately 15 genera are known, and most of the hyperthermophilic species have been isolated from marine or terrestrial volcanic environments, such as hot springs and shallow or deepsea hydrothermal vents. Recent analyses of genetic sequences obtained directly from environmental samples, however, indicate the existence of low temperature Crenarchaeota, which have not yet been cultivated. The most spectacular fea ture of the Crenarchaeota, however, is their tolerance Substrates and bacterial groups involved in methane production (After Christen and Kjelsen 1989) of, and even preference for, extremes of acidity and temperature. While many prefer neutral to slightly acidic pH ranges, members of the Crenarchaeal order Sulfolobales flourish at pH 1-2 and die above pH 7. Optimum growth temperatures range from 75°C to 105°C and the maximum temperature of growth can be as high as 113°C (Pyrobolus). Most species are unable to grow below 70°C, although they can survive for long periods at lower temperatures. Crenarchaeota contains representations of organisms which live in a wide variety of environments including terrestrial environ ments (hot springs, geothermal power plants) or in marine (submarine hot vents, deep oil wells, marine smokers up to 400°C). Some exist in environments of over 100°C, while others live at ice cold conditions. For substrates, they utilize a wide range of gases: CO 2 , CO, CH 4 , S 2 O 3 , N 2 , NH 4 (Fig. 4.19) . Temperatures as high as 100°C occur around ter restrial volcanoes and Sulfolobus and Thermoproteus, both hyperthermophiles, have been isolated from such environments. Archae with the highest optimum temperature of growth known occur in underwater vents and near underwater volcanoes. Pyrodictium sp. and Pyrolobus sp. have optimum temperatures of growth of 100°C and 106°C respectively and are found in such environments. Desulforococcus (90°C, optimum) and Staphylothermus (95°C, optimum) are also found in that environment. The Domain Eukarya includes plants, animals, algae, fungi, and protozoa. The last three are regarded as microorganisms, although some of them are quite large. In Fig. 4 Fig. 4.19 Phylogenetic tree of the Archae (Modified from Ciccarelli et al. 2006) Note: The genera of Archeae are given above. They are placed in the two phyla of Archeae which have been cultivated, Euarchaeota and Crenarchaeota. A third phylum, the Korarcheota are only known from their DNA sequences and have not yet been cultivated. The notations in red are orders in which the genera are grouped. Thus the halophilic archeae are grouped among the Halobacteriales the methane producers are in Methagenales Protozoa are classified in many ways, primarily on morphological characteristics, and the one adopted here groups them into five: Mastigophora, Sarcodina, Ciliata, Sporozoa, and Suctoria. 1. Flagellata (Mastigophora) These possess flagella and are subdivided into "phyto flagellata" and "zooflagellata," depending on whether they are plantlike (with chlorophyll) or animallike (without chlorophyll). They usually multiply by lon gitudinal binary fission. Many flagellates are able to feed autotrophically as well as heterotrophically, and are important primary producers in lakes and oceans; yet, they can also feed like animals, ingesting or absorbing food synthesized by other organisms. Many are freeliving, but some are parasitic. Examples of parasitic Mastigophora are Trypano soma gambiense and T. rhodesiense which cause African sleeping sickness and is transmitted by tsetse flies. T. cruzi is the cause of Chagas' disease, prevalent in South and Central America, which affects the nervous system and heart; it is transmit ted by the bite of assassin bugs. Giardiasis is caused by the mastigophoran Giardia lamblia. These Protozoa use pseudopodia (false feet) for locomotion and for catching preys. Members of the group Sarcodina move by pseudopodia; although, flagella may be present in the reproductive stages. Cytoplasmic streaming assists movement. Asexual reproduction occurs by fission of the cell. Sarcodina includes two marine groups known as foraminiferans and radiolarians. Both groups were present on earth when the oil fields were in formative stages, and marine geologists use them as potential markers for oil fields. Some amoebae live in shells from which the pseudopodia are extruded. Some members of the group such as Entamoeba histolytica, are pathogenic, causing amoebic dysentery in humans. This organism can cause painful lesions of the intes tine and is contracted in polluted water (Fig. 4.21) . Ciliates possess cilia (short and highly coordinated flagellae), a somatic (macro) nucleus, and genetic (micro) nucleus, and a contractile vacuole is usually present. They move by means of cilia. Conjugation may be used for sexual reproduction and binary fis sion also occurs. The distinctive rows of cilia vibrate in synchrony and propel the organism in one direc tion. One of the best known members of the group is Paramecium; another of the freeliving members of this group, is Tetrahymena. Ciliates form an extremely large group are dis tinguished by the possession of cilia, two different types of nuclei and transverse fission of the organ ism when it divides, unlike flagellates and sarcodina which divide longitudinally. Members The juvenile forms are ciliated and motile, while the adult forms are sessile and capture food by tentacles. They feed by extracellular digestion and lack cilia in the adult phase. The adult have structures called hap tocysts at the tip which attach to the prey. The prey's cytoplasm is then sucked directly into a food vacuole inside the cell, where its contents are digested and absorbed. Most suctoria are around 15-30 mm in size, with a noncontractile stalk and often a shell. Suctoria reproduce primarily by budding, producing swarmers which lack both tentacles and stalks but have cilia. Once the swarmers (motile young) have found a place to attach themselves, they quickly develop stalks and tentacles and lose their cilia. Because of the presence of cilia in the young of suctoria, some authors group the suctoria among ciliates. Suctoria are found in both freshwater and marine environments, and some which live on the surface of aquatic animals, and typically feed on ciliates. Some marine species form symbiotic rela tionships with crustaceans and even some fish. One species, Ephelota gemmipara lives on the external parasite of salmon, Lepeophtheirus sal monis (salmon louse). Fungi are eukaryotic microorganisms which (a) Are nonphotosynthetic and hence do not contain chlorophyll (b) Contain chitin and/or cellulose in their cell walls (c) Are usually filamentous (called molds), but they may be unicellular (called yeasts) (d) Reproduce asexually with spores The classification of the fungi is based mainly on morphology of the hyphae, the structures housing the sexual structures, or the structure to which the sexual spores are attached (Samson and Pitt 1989; Guarro et al. 1999) . The principal diagnostic characteristics are shown in Fig. 4 Table 4 .8). An ascus or sac (plural, asci) which contains ascosposcores (sexual spores typically eight in number housed in an ascus) is diagnostic of Ascomycetes (Ascomycota). The trivial name of this group of fungi is sac fungi. The presence of basidiospores, typically four in number attached to a basidium, (a clublike struc ture) identifies Basidiomycetes. Some of the best known Basidiomycetes (Basidiomycota) are mush rooms. A microscopic examination of the "gills" on the underside of the mushrooms reveals the basidia carrying the basidiospores. Algae are photosynthetic eukaryotic organisms which lack the structures of vascular plants. Many authors classify them as microorganisms, but they are highly variable in size and range from microscopic sizes to the brown algae which could be up to 70 m long (Trainor 1978; Sze 1986) (Fig. 4.24) . The classification of the algae is based on the following: (a) Pigmentation The various kinds of pigments in the algae, as well as the overall color of the alga, are used in classifying the organisms. All of the groups contain the follow ing pigments which are soluble in organic solvents: Chlorophylls and several carotenoids, which include carotenes and xanthophylls. Chlorophylls "a" and "b," alpha or beta carotene, and some xanthophylls are common. The water soluble phycobiliproteins (phycobilins) are found in bluegreen algae, red algae, and a small group of flagellates. Reserve food material is usually stored within the cell and frequently within the plastid in which photosynthesis occurred. Starch, starchlike com pounds, fats, or oils are the most common forms. (c) The nature of the zoospores Some organisms are motile during much of their lives, whereas other genera lack motility, or any motile reproductive stages. Adult algae are usually nonmotile; often, however, some reproductive stages (zoospores) are motile. The overall shape of the zoospores, the shape, number, and the insertion position of the flagella, and the presence or absence of hairs on the flagella are diagnostic (Fig. 4.24 ; Table 4 .9). The cell wall may be a simple outer covering around the protoplast or an elaborately ornamented struc ture. The materials found in algal walls are cellulose, xylans, mannans, sulfated polysaccharides, alginic acid, protein, silicon dioxide, and calcium carbonate (e) Gross morphology of the alga The overall shape of the alga is diagnostic. The various groups of algae are given in the Table 4 .9. Fig. 4 .24 Illustrations of some algae (All items in the table reproduced with permission) a) Red algae are red because of the presence of the pigment phycoerythrin; this pigment reflects red light and absorbs blue light. Because blue light penetrates water to a greater depth than light of longer wavelengths, these pigments allow red algae to photosynthesize and live at somewhat greater depths than most other algae. The picture of the red alga, Dichotomaria marginata, shown here was taken and kindly supplied by Keoki Stender, University of Hawaii. b) Sargassum fluitans. Sargassum seaweed, Gulf Weed (brown alga). This is a major component of the algae in the Sargasso Sea in the pelagic Atlantic. It has long, serrated fronds with a distinctive midrib, and smooth berrylike spherical gasfilled bladders, pneumatocysts, which assist the floatation of the alga.The photo of Sargassum above was kindly supplied by the South Carolia Department of Natural Resource, courtesy of H. Scott Meister. c) Synura spp, a member of the Chrysophyceae (golden or goldenbrown algae on account of their content of fucoxanthin which in the presence of chlorophyll makes them look brown or golden brown), forms swimming colonies from a variable number of cells joined together at their posterior ends in a spherical or elongated cluster. Synura is important because it gives drinking water a bitter taste and a "fishy" cod liver oil type of odour. Synura is freshwater; some marine members such as Olisthodiscus luteus, produce neurotoxins which may kill aquatic fauna and may affect humans through eating shell fish raw. Credit: Dr Graham Matthews, graham@gpmatthews.nildram.co.uk (http://www. gpmatthews.nildram.co.uk/microscopes/pondlife_plants01.html). Dr Graham Mathews is also Hon Secretary of the Secretary of the Quekett Microscopical Club) d) Bacillaropyceae (Diatoms) are one of the largest and ecologically most significant groups of organisms on Earth. Diatoms are microscopic algae which are easily recognizable because of their unique cell structure, silicified cell wall and life cycle. Diatoms are found anywhere there is water and light: in oceans, lakes and rivers; marshes, fens and bogs; damp moss and rock faces. They are an important part of the food chain in aquatic environments, especially in nutrient-rich areas of the world's oceans, where they occur in abundance.Photograph of diatoms kindly supplied by Dr David Carling) e) Dinoflagellates are minute marine unicellular algae with diverse morphology, the largest, Noctiluca, being as large as 2 mm in diameter!. Many are photosynthetic, while some are parasites of fish. In temperate climates they form blooms in summer months which may be golden or red. Their blooms produce neurotoxins marine animals eating and humans who consume them raw (such as shellfish) Until recently, viruses were not thought to be abundant or important in the aquatic environment. We now know that they are not only abundant, but that they pro foundly influence the ecology and food status of the aquatic environment including seas and oceans. Viruses are lifeless crystals of nucleic acid which are able to grow and reproduce only in living cells. They differ from cells in the following ways, and also have the following properties: 1. Whereas cells contain both DNA and RNA, viruses contain either DNA or RNA, never both. and outer protein cover, the capsid (see Fig. 4 .26). 3. Viruses enter only susceptible cells: thus there are viruses which will attack only plants while some will attack only animals. Even among plants and animals, some viruses will attack some members and not the others. 4. All living things are attacked by viruses, including the microorganisms: Bacteria, fungi, algae, and protozoa. Viruses attacking bacteria and fungi are bacteriophages and mycophages, respectively. Viruses used to be classified on their diseases they cause and their sizes and shapes, but these criteria have The nomenclature of viruses is based on a set of rules set up by the International Committee on the Taxonomy of Viruses (ICTV), which since the 1960s has been arranging viruses in these seven groups into taxonomic hierarchies. The criteria for the taxonomic arrangements are: 1. Morphology (Helical, e.g., bacteriophage M13; icosohedral/poly hedral/cubic, e.g., poliovirus, enveloped -may have poyhedral (e.g., herpes simplex) or helical (e.g., influenza virus) capsids, complex, e.g., pox viruses) 2. Nucleic acid type, 3. Whether the virus is naked or enveloped 4. Mode of replication 5. Host organisms 6. The type of disease they cause Viral taxonomic nomenclature is modeled after that of cellular organisms. However viruses suffer from the absence of fossil record which will enable more phylo genetic relationships among the various groups. Consequently, the highest level in the viral taxonomic hierarchy is the order, thus: Order ( Note that the HIV 1 virus has an envelope (matrix in the dia gram above). Not all viruses have envelopes; those which do not are said to be naked (see text). The gp structures are glycoprotein. (Retroviral) integrase is an enzyme produced by a retrovirus that enables its genetic material to be integrated into the DNA of the infected cell. Note also the reverse transcriptase (produced by retroviruses such as HIV), a DNA polymerase enzyme that tran scribes singlestranded RNA into doublestranded DNA The names of virus orders, families, subfamilies, • genera, and species should be written in italics with the first letter capitalized. Other words are not capitalized unless they are • proper nouns, e.g., Tobacco mosaic virus, Poliovirus, Murray River encephalitis virus. This format should only be used when official taxo • nomic entities are referred to it is not possible to centrifuge the species, for example, Poliovirus, but it is possible to centrifuge poliovirus. Italics and capitalization are not used for vernacular • forms (e.g., rhinoviruses, c.f. the genus Rhinovirus), for acronyms (e.g., HIV1), nor for adjectival usage (e.g., poliovirus polymerase). ), Poxviridae (smallpox), and many tailed bacteriophages. The mimivirus is also placed into this group (see Table 4 .10). Group II: These viruses possess singlestranded DNA and include such virus families as Parvoviridae and the important bacteriophage M13 (see Table 4 .11). Group III: These viruses possess doublestranded RNA genomes, e.g., rotavirus. These genomes are always segmented. Segmented virus genomes are those which are divided into two or more physically separate molecules of nucleic acid, all of which are then packaged into a single virus particle (see Table 4 .12). Group IV: These viruses possess positivesense single stranded RNA genomes. Many well known viruses are found in this group, including the picornaviruses (which is a family of viruses that includes wellknown viruses like Hepatitis A virus, enteroviruses, rhinovi ruses, poliovirus, and footandmouth virus), SARS virus, hepatitis C virus, yellow fever virus, and rubella virus. Positivesense viral RNA is identical to viral mRNA and thus can be immediately translated by the host cell (see Table 4 .13). Group V: These viruses possess negativesense single stranded RNA genomes. The deadly Ebola and Marburg viruses are well known members of this group, along with influenza virus, measles, mumps, and rabies. Negativesense viral RNA is complemen tary to mRNA and thus must be converted to positive sense RNA by an RNA polymerase before translation (see Table 4 .14). Table 4 .16. The structures of the various viruses whether they are DNA or RNA are highly variable. The structure of the DNA viruses are shown in Table 4 .17 and those of the RNA viruses are shown in Table 4 .18. Until recently, it was thought that aquatic environ ments, marine and freshwater, were devoid of viruses. New techniques now show them to be abundant in the aquatic environment, where they contribute to nutrient cycle by lysing microorganisms. All microorganisms, bacteria (bacteriophages), fungi (mycophages), algae (phycophages), and protozoa are attacked by viruses (phages, phago = eat, Greek) which attack (eat) them. Bacteriophages are the most abundant among the phages and they have been more widely studied. Bacteriophages were first formally described by the French Canadian Felix d' Herelle in 1915, but the ini tial observations were made during 1896, followed by observations made by the British bacteriologist Frederick Twort in 1913 (see Fig. 4.26) . On account of their importance in aquatic systems, the life cycle of bacterial viruses, the methods of isolating and enumer ating them from water, their grouping, and their host range will be discussed below. When bacteriophages enter susceptible bacteria, they take over the genetic apparatus of their hosts and force the hosts to produce more viruses of their type. When the virions (virus particles) mature, they produce enzymes which lyse the host cell wall releasing the virus particle to start life afresh. When they lyse the host they are in the lytic phase. Sometimes they enter into a phase, the lysogenic phase, in which the phages remain in the cell and replicate with it. This phase is the lysogenic phase (see Fig. 4 .27). Because of their small size, bacteriophages are not usually studied directly as is the case with microorganisms. An electron microscope is necessary to study viruses, but not only are electron microscopes expensive, but they require skilled operators to handle them. Therefore, viruses are studied indirectly through their effects. The indirect meth ods used especially for animal and plant viruses, include the changes (known as cytopathic effects, CPE) they bring about in the cells in the cell culture in which they are grown: lysis, altered shape, detachment from substrate, membrane fusion, altered membrane permeability. Other methods for studying viruses, particularly of animals and plants, are serological methods based on the interaction between virus and antibody produced specifically against it, detection of viral nucleic acid, including the use of polymerase chain reaction (PCR) for the detection of DNA or RNA. These methods are used mostly for studying animal and plant viruses. For bacteriophages, the chief method of detection is the cytopathic effect (CPE). Bacteriophages are sometimes very abundant in water and because of the specificity of the bacteria they attack, it has been suggested that they can be used as indicators of fecal pollution of water. Bacteriophages may be isolated and/or enumerated from water in the following ways (McLaughlin et al. This method is used if the aim is to isolate phages attacking a particular bacterium from the water sam ple. A pure culture of the bacterium whose phages are to be isolated is introduced into sample of the water to be assessed for phage load, say about 1 ml of a log phase culture of the bacterium is added to about 10-15 ml of the water and incubated under conditions which will encourage the growth of the bacterium, including shaking if necessary. At the end of 18-24 h growth, a quantity of chloroform is added to kill the bacteria, and the broth is filtered in a 0.45 mm filter to remove the debris. The filtrate is then serially diluted and about 0.5-1 ml of the dilu tions mixed with molten agar at 45°C and poured in to plates and incubated. It is assumed that each zone of clearing (plaque) on the bacterial lawn indicates one bacteriophage, or more correctly, one plaque forming unit (PFU), since as the case with bacteria, a clearing could be formed by a clump of bacterio phages. To ensure the avoidance of clumps, the counting or selection should done with as high a dilution as possible; the filtrate can also be shaken to breakup clumps before introduction into the agar. Some workers prefer to use the soft agar method. In this method, a small volume of a dilution of phage suspension and a small quantity of host cells grown to high cell density, sufficient to give 10 7 -10 8 CFU/ml (colony forming units/ml), are mixed in about 2.5 ml of molten, "soft" agar at 46°C. The resulting suspension is then poured on to an appro priate basal agar medium. This poured mixture cools and forms a thin "top layer" which hardens and immobilizes the bacteria. If the aim is to assess the diversity of phages present in the water body, several dilutions of the water are made. At each dilution, pour plates are made as described above, each plate with one of the variety of bacteria whose phages are being sought in the water. (c) Direct counting in a flow cytometer In this method, the water may be centrifuged to concentrate the virus. The phages are stained with highly fluorescent nucleic acid specific dyes such as SYBR Green I, SYBR Green II, OliGreen, or PicoGreen. Flow cytometry allows extremely rapid enumeration of single cells, primarily by optical means. Cells scatter light when passing through the laser beam and emit fluorescent light when excited by the laser. Flow cytometry has become an invaluable tool for both qualitative and quantitative analyses owing to its rapidity. It has been used as a rapid method for detecting viruses from different families. Flow cytometry appears faster and more accurate than any other method currently used for the direct detection and quantification of virus particles (Brussaard et al. 2000) . Although epifluorescence microscopy is commonly used for the enumeration of bacteria and other micro organisms in natural water samples including viruses, because of its simplicity and ready availability of the microscopes, distinguishing viruses based on differ ences in fluorescence intensity is difficult with the epifluorscence microscope; small bacteria may for example be counted for large viruses. Figure 4 .28 gives the names of the bacteriophages, the description of their virions and the hosts which they attack. It will be seen that in many cases, the same bac teriophages may sometimes attack numerous hosts, while in some cases, a bacteriophage is restricted to one host. Two groups of small multicellular macroorganisms occur in water, namely, crustaceans (including rotifers) and nematodes. Phages consist of a capsid and an internal lipid membrane. Virus capsid is not enveloped. Internal lipid membrane located between outer and inner protein shell. Capsid/nucleocapsid is round and exhibits icosahedral symmetry (T=12), or 13). The capsid is iso metric and has a diameter of 60 nm (or more). The capsid shells of virions are composed of three layers. Capsids appear hexagonal in outline. The capsid surface structure reveals a regular pattern with distinctive features. The capsomer arrangement is clearly visible. Surface projections are distinct, brushlike spikes protruding from the 12 vertices. Capsids all have the same appearance. The genome is not segmented, constitutes 13% of the virus's weight and contains a single molecule of circular, supercoiled, double-stranded DNA of 9500-12000 nucleotides in length. The genome has a g + c content of 43%. Their hosts are members of the Phylum Proteobacteria. Members of the Cystoviridae appear to be most closely related to the Reoviridae but also share homology with the Totiviridae. Cystoviruses are the only bacteriophage that are more closely related to viruses of eukaryotes than to other phage. Most identified cystoviruses infect Pseudomonas species, but this is likely biased due to the method of screening and enrich ment. The type species is Pseudomonas phage F6, but there are many other members of this family. F7, F8, F9, F10, F11, F12 and F13 have been identified and named, but other cystovi ruses have also been isolated. The genome of a fuselloviridae is nonsegmented and con tains a single molecule of circular, doublestranded DNA. The DNA is positively supercoiled. The complete genome is 15500 nucleotides in length; encodes for 31 to 37 genes. Fuselloviridae virions consist of an envelope and a nucleo capsid. The capsid is enveloped. Virions are spindleshaped, flexible, and have protrusions that extend through the envelope. One pole has short taillike fibers attached to it. The virions are 100 nm in length and 60 nm in diameter. Fuselloviridae infect the Archae Sulfolobus which inhabits high-temperature (>70°C), acidic (pH of <4.0) environments. Members of this family have been found in acidic hotsprings in Japan and Iceland. The Fuselloviridae family currently consists of only one virus, Sulfolobus spindleshaped virus 1 (SSV1), and three tentative members (SSV2, SSV3, and the staaelite virus pSSVx, which stands for plasmid SSV x). SSV1, the type virus for the family, was the first hightemperature virus to be characterized. Members of the family infect their natural hosts without causing lysis, and the infected cells continue to divide and produce virus indefinitely. The hosts are plant and animal pathogens. In several systems the phage enter into lysogenic phases. lnouirus hosts are all gramnegative bacteria (i.e., Escherichia coli, Salmonella, Pseudomonas, Vibrio, Xanthomonas, etc.) . Host ranges are determined primarily by host cell receptors, which are usually conjugative pili. Some pili are encoded chro mosomally and some are encoded on plasmids of different incompatibility groups. Transmission of the plasmids to new bacterial species usually transfers phage sensitivity. Additional host range determinants include restrictionmodification sys tems, host periplasmic proteins involved in viral ssDNA translo cation into the cytoplasm, and host protein(s) involved in membrane assembly. Transfections of nonnatural hosts with naked ssDNA or dsDNA are sometimes possible. When Vibrio cholera phage lysogens colonize the human intestine, states of elevated cholera toxin expression and release, and of progeny filamentous choleraphage extrusion, are induced. Thus lnaoirus lysogeny is a critical virulence factor in cholera pathogenesis. Non-enveloped, spherical virion about 26nm in diameter with icosahedral symmetry (T=3) composed of 180 CP proteins and a single A protein. Linear, ssRNA(+) genome about 4 kb in size. The 5' end is capped. Encodes for 4 proteins. It attacks Enterobacteriacea, Acinetobacter, Caulobacter and Pseudomonas. Enveloped, rod-shaped. The capsid is about 24-38 nm in diam eter and 410-1950 nm in length. Linear dsDNA genome of 15.9 to 56 kb. Extremities of the DNAare modified in an unknown manner. The Lipothrixviridae family consists of a family of viruses that infect archaea. They share characteristics from the Rudiviridae family and both have are filamentous viruses with linear dsDNA genomes that infect thermophilic archaea in the kingdom Crenarchaeota. Lipothrixviridae are enveloped. Lipothrixviridae is a family crenarchaeal viruses. It is by far the most diverse family of crenarchaeal viruses, with six isolates divided into three genera: Alphalipothrixvirus, Betalipothrix virus, and Gammalipothrixvirus. Alphalipothrixvirus contains TTV1, TTV2, and TTV3, isolated from acidic hot springs Iceland. Betalipothrixvirus contains SIFV, also isolated in Iceland. Finally, Gammalipothrixvirus is represented by AFV1, isolated from Yellowstone National Park. Also Acidianus, Sulfolobus, Thermoproteus. Myoviruses are not enveloped and consist of a head and a tail sepa rated by a neck. The head has icosahedral symmetry, while the tail is tubular and has helical symmetry. The capsid that constitutes the head is made up of 152 capsomers. The head has a diameter of 50-110nm; the tail is 16-20nm in diameter. The tail consists of a central tube, a contractile sheath, a collar, a base plate, six tail pins and six long fibers. Tail structure is similar to tectiviridae, but dif fers in the fact that a myovirus' tail is permanent. Contractions of the tail require ATP. When the sheath is contracted, it measures 1015 nm in lengthicosahedral capsid, circular ssDNA. Myoviruses, being bacteriophages, infect bacteria. The most com monly infected bacteria is Escherichia coli. Myoviruses are viru lent phages, meaning they do not integrate their genetic material with their host cell's, and they usually kill their host cell. Others are Bdellovibrio, Chlamydia, Enterobacteria, Spiroplasma. Pleomorphic, envelope, lipids, no capsid, circular supercoiled dsDNA. Enveloped, spherical to pleomorphic, no headtail structure. The capsid is about 80 nm in diameter. The Plasmaviridae is a family of bacteriophages, viruses that infects bacteria. Virions have an envelope, a nucleoprotein com plex, and a capsid. They are 50-125 nm in diameter with a baggy or loose membrane. The genome is condensed, non segmented and consists of a single molecule of circular, supercoiled doublestranded DNA, 12000 base pairs in length. The genome has a rather high G-C content of around 32 percent. A productive infectious cycle begins before a lysogenic cycle establishes the virus in the infected bacteria. After initial infection of the viral genome the virus may become latent within the host. Lysogeny involves integration into the host chromosome. A wellknown host is Acholeplasma. Nonenveloped, headtail structure. Head is about 60 nm in diam eter. The tail is noncontractile, has 6 short subterminal fibers. The capsid is icosahedral with a T=7 symmetry. It has a linear, dsDNA genome of about 40-42 kb encoding for 55 genes. Wide range of bacterial hosts including Gram positive and Gram negative. Nonenveloped, rodshaped, rigid, with three tail fibers at either end. Linear dsDNA genome of 32-35 kb. At both ends, there are inverted terminal repeats as well as seven direct repeats. The two strands of the linear genomes are covalently linked. Wide range of bacteria, Gram positive and Gram negative. Siphoviridae are a family of doublestranded DNA viruses infecting only bacteria that are characterized by a long noncon tractile tail and an isometric capsid (morphotype B1) or a prolate capsid (morphotype B2). The Siphoviridae viruses have a capsid with a diameter of about 5560 nm and a long tail that can reach up to 570 nm. Their doublestranded DNA is linear. Nonenveloped, headtail structure. The head is about 60 nm in diameter. The tail is noncontractile, has fibers, and is fila mentous. The capsid is icosahedral with a T=7 symmetry. Linear, dsDNA genome of about 50 kb, containing about 70 genes. Wide range of bacteria, Gram positive and Gram negative. Non enveloped, icosahedral virion with a pseudo T=25 symmetry. Virion size is about 66 nm with apical spikes of 20 nm. The capsid encloses an inner membrane vesicle within which the genomic DNAis coiled. Linear, dsDNA genome of about 15 kb flanked by inverted repeats. Encodes for 30 ORFs. Replication is proteinprimed. A wide range of bacteria including Alicyclobacillus, Bacillus, Enterobacteria, Pseudomonas, Thermus. Microscopic crustaceans like tiny lobsters are found in sewage works where they feed on bacteria and algae. Some of the species encountered are Cyclops spp., Paracyclops spp., and Oaphia spp. Rotifers, small microscopic animals of the class Rotifera, are found in water in great abundance. They are usually less than 1 mm, most usually in the range of 500 mm in length. Three orders are known: Seisonidae is marine, while the other two, Bdelloidea and Monongononta, are freshwater and found in reser voirs, streams, and sewage treatment plants. Rotifers may be sessile or planktonic, although they can swim with their cilia; their usual locomotive method is by crawling. They are common in structures with large exposed surfaces such as in trickling filters sewage treatment plants. They are found in oligotrpic waters, i.e., waters low in organic matter, for example in sewage effluents and reservoirs after protozoa have died off, and thus are indicators of posteutrophication waters. Indeed, they have been used as indicators of water quality. Various species are identified with dif ferent levels of water quality. Brachionus angularis, Trichocerca cylindrica, Polyurthra euryptera, Pompholyx sulcata, Rotaria rotatoria, Filinia long iseta have been designated as indicators of heavy pol lution (eutrophic) while Ascomorpha ovalis, Asplanchna herricki, Synchaeta grandis, Ploesoma hudsoni, Anuraeopsis fissa, Monostyla bulla, and M. hamata are indicators of fresh and clean waters (olig otrophic). A variety of rotifers including Brachionus, Keratella spec, are inhabitants of moderately clean (mesotrophic) waters (Saksena 2006) . Rotifers have been also been used to detect the oocysts of Cryptosporidium, in water samples. The fluorescent insitu hybridization (FISH) technique (see Sect. 4.1.3.3.2d) applied to rotifers has enabled the detection of biological contamination of surface water through an assessment of the dispersive stages of the parasite (see Table 4 .19). Other crustaceans found in water are Daphnia, Cyclops, Synchaeta. Nematodes are invertebrate roundworms that inhabit marine, freshwater, and terrestrial environments. They comprise the phylum Nematoda (or Nemata) which includes parasites of plants and of animals, including humans, as well as species that feed on bac teria, fungi, algae, and on other nematodes. Four out of every five multicellular animals on the planet are nematodes. The majority of nematodes are micro scopic, averaging less than a millimeter in length, but some of the animal parasites are quite large and read ily visible to the naked eye. Nematodes that feed on other organisms are important participants in the cycling of minerals and nutrients in the ecosystem that is fundamental to other biological activity. Some of these nematodes may have major roles in decom position, including biodegradation of toxic com pounds. In fact, the incidence of certain nematode species is sometimes used as an indicator of environ mental quality (Fig. 4.29) . Nematodes are, by nature, aquatic organisms. It is estimated that about 50% of nematode species inhabit marine environments, although many of these have yet to be described and characterized. The remainder of the species inhabit soil and freshwater. In the soil, their aquatic requirements are satisfied by inhabiting the water films around soil particles. Parasitic nematodes are bio logically active when bathed in moisture films supplied by water in the tissues or body fluids of the host. Nematodes in freshwater aquatic systems also serve as a nutrient source for invertebrates, small vertebrates, and fungi. The source of food for these nematodes is pri marily bacteria, but algae and fungi are also consumed. The marine environment provides habitat for an enormous diversity of nematodes, from surface, littoral, and estuarine zones to the ocean depths. One interest ing group of deep sea nematodes are the Rhaptothyridae, which have no mouth and a very reduced alimentary tract. The digestive tract is filled with symbiotic chemoaototrophic bacteria. A similar relationship exists in the mouthless genus Astomonema. Nematodes are widely distributed in aquatic and soil habitats and are particularly common in waters rich in organic matter such as sewage. 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