key: cord-0931393-ifgfzcsl authors: Müller, Marcel A.; Paweska, Janusz T.; Leman, Patricia A.; Drosten, Christian; Grywna, Klaus; Kemp, Alan; Braack, Leo; Sonnenberg, Karen; Niedrig, Matthias; Swanepoel, Robert title: Coronavirus Antibodies in African Bat Species date: 2007-09-03 journal: Emerg Infect Dis DOI: 10.3201/eid1309.070342 sha: 5bb307428f45e725c931894d2ed7d06d7f8d0991 doc_id: 931393 cord_uid: ifgfzcsl Asian bats have been identified as potential reservoir hosts of coronaviruses associated with severe acute respiratory syndrome (SARS-CoV). We detected antibody reactive with SARS-CoV antigen in 47 (6.7%) of 705 bat serum specimens comprising 26 species collected in Africa; thus, African bats may harbor agents related to putative group 4 CoV. Bat serum specimens (n = 705) collected from 1986 through 1999 in South Africa (SA) and the Democratic Republic of the Congo (DRC) were tested. The fi rst 248 serum specimens were collected from 1986 through 1989 in the Mpumalanga and Limpopo Provinces of SA for studies on rabies-related viruses, with the approval of the provincial Directorates of Nature Conservation and the Animal Ethics Committee of the University of the Witwatersrand. The remaining 457 serum samples were collected in 1995-1999 in the Bandundu and Oriental Provinces of the DRC for studies on Ebola and Marburg viruses, under the auspices of the International Committees for the Control of Ebola hemorrhagic fever in Kikwit, and Marburg hemorrhagic fever in Durba-Watsa, coordinated by the World Health Organization on behalf of the government of DRC. Bats were caught in mist nets, anesthetized, and exsanguinated by cardiac puncture. Serum specimens were stored at -70°C until analyzed. For screening of serum specimens we used the SARS-CoV ELISA kit (EUROIMMUN AG, Lübeck, Germany) with minor modifi cations. Bat serum samples were tested at a dilution of 1:50, and horseradish peroxidase-labeled goat antibat immunoglobulin (Ig) conjugate (Bethyl, Montgomery, AL, USA) was used as secondary antibody at a dilution of 1:2,000. Negative bat serum was obtained from a captive-bred Rousettus aegyptiacus at the National Institute for Communicable Diseases, Sandringham, SA. The cutoff was determined as 3× the mean optical density value at 450/605 nm observed in negative control samples. Positive serum samples were retested and their titers determined. To evaluate test specifi city and to exclude possible crossreactivity to other viruses, especially to HCoVs, which have a seroprevalence in humans >90% (11) , 662 human serum specimens were screened (online Technical Appendix, available from www.cdc.gov/EID/content/13/9/1367-Techapp.htm), including those from 90 patients with other acute respiratory infections, 70 HCoV-229E-positive serum specimens and 4 HCoV-NL63-positive serum specimens (provided by L. van der Hoek). A confi rmatory Western blot (WB) was done by using protein lysates from Vero E6 cell cultures (American Type Culture Collection [Manassas, VA, USA] CRL 1586) infected with SARS-CoV Hong Kong isolate 6109 (Gen-Bank accession no. AY278491) and from uninfected Vero E6 cultures. Bat serum specimens were applied at dilutions of 1:500 and 1:2,000. Secondary detection was performed with the SuperSignal West Dura Extended Substrate chemiluminescence detection assay (Pierce Biotechnology, Rockford, IL, USA). The signal intensity of the 150-kDa spike (S), 50-kDa nucleocapsid (N) proteins was evaluated independently by 2 operators. For a second confi rmatory WB, recombinant SARS-CoV proteins were used. For prokaryotic expression of recombinant SARS-CoV N protein and a fragment of the S protein (amino acid positions 318-510), we followed the instructions of the Champion pET Directional TOPO Expression kit (Invitrogen, Karlsruhe, Germany) using plasmids pET101-N and pET102-Saa318-510. Purifi cation and refolding of the protein on column were done as described previously (12) . Purifi ed recombinant protein (15 μg) was resolved by electrophoresis on a discontinuous 12% sodium dodecyl sulfate-polyacrylamide gel. After blotting, nitrocellulose strips were incubated with bat serum samples diluted 1:2,500 and 1:5,000. One positive bat serum specimen was used as a reference to exclude *Robert Koch-Institut, Berlin, Germany; †National Institute for Communicable Diseases, Sandringham, South Africa; ‡Bernhard Nocht Institute for Tropical Medicine, Hamburg, Germany; §Conservation International, Cape Town, South Africa; and ¶EUROIMMUN AG, Lübeck, Germany variations in experimental procedures and signal intensities. Serum specimens that produced signals at a dilution 1:5,000 were considered positive as none of the control serum specimens showed reactivity at that dilution. To evaluate assay specifi city, we tested 19 control serum specimens comprising 12 randomly selected bat serum specimens that were negative by ELISA, 2 SARS-CoV-positive human serum specimens, and 5 SARS-CoV-negative human serum specimens, including 4 HCoV-NL63-positive serum specimens. A commercial indirect immunofl uorescence test (SARS-CoV-IFTII kit, EUROIMMUN AG) was carried out as described by the manufacturer, except that bat serum samples were diluted 1:100, and slides were incubated at room temperature for 2 hours. Reactions were detected with goat-antibat immunogolublin (Ig) (Bethyl) at a dilution of 1:1,000 and fl uorescein isothiocyanate-labeled donkey-antigoat Ig (Dianova, Hamburg, Germany) at a dilution of 1:100. Specifi city of the indirect immunofl uorescence test (IIFT) was determined by screening 572 human serum specimens. The sensitivity and correlation of IIFT versus ELISA were analyzed (online Technical Appendix). In addition, the 19 selected control serum samples were tested. Virus neutralization tests were performed as described elsewhere (13) except for using Vero E6 cells cultured in Dulbecco's modifi ed Eagle medium and SARS-CoV Hong Kong isolate 6109 (3.25 × 10 7 PFU/mL, diluted 1:5,000). Bat serum dilutions in quadruplicate ranged from 1:10 to 1:320. After incubation at 37°C in 5% CO 2 for 3 days, the cells were fi xed with 8% formaldehyde and results interpreted as described (13) . Viral RNA was extracted from serum by using a QIAamp viral RNA extraction kit (QIAGEN, Hilden, Germany), and reverse transcription-PCR (RT-PCR) was performed essentially as described elsewhere (14) , with the exception that 140 μL was not available from every bat. In such cases, input volume was reduced and replaced with water. A minimum of 20 μL was usually tested. Antibody activity to SARS-CoV antigen was detected by ELISA in 7 of 26 bat species tested at both collection sites with a seroprevalence of 6.7% (47/705). The highest prevalences were found in the fruit bat Rousettus aegyptiacus (Chiroptera: Pteropodidae) (16.4%) and the insectivorous bat Mops condylurus (Chiroptera: Molossidae) (12.2%) (Table) . ELISA titers ranged from 50 (73% of the serum samples) to 800. Confi rmatory WB analyses performed by 2 methods on ELISA-positive samples for which suffi cient material remained available, were positive in 36 (97.3%) of 37 serum specimens, but IIFT was positive in only 12 (32.4%) of 37 samples (Table; Figures ; Figures 1, 2) . Neutralizing activity to SARS-CoV was not found in any of the ELISA-positive samples, and RT-PCR did not detect CoV nucleic acid in 262 serum specimens tested (data not shown). The results of WB analyses support the specifi city of the ELISA used in this study. The IF test is known to be less sensitive than ELISA but still provided confi rmation in one third of the serum specimens tested. The negative results in the viral neutralization tests are not unexpected because this assay detects only antibodies that interfere with the specifi c entry mechanism of SARS-CoV, and putative group 4 CoVs from African bats may not use it. Moreover, deletions and mutations found in Asian bat SARS-like-CoV isolates lie in the S protein region essential for binding of SARS-CoV to the cellular receptor, angiotensin-converting enzyme 2, and thus are likely to affect cross-neutralization, as emphasized by confl icting results obtained in Asia (6, 7, 15) . The negative fi ndings obtained in RT-PCR can be explained by the unlikelihood of fi nding virus nucleic acid in serum. Studies in Asia used rectal swabs instead of serum samples, and the virus likely persists in the enteric tract but may not be found in serum at all. Both bat species (R. aegyptiacus and M. condylurus) are widely distributed in Africa but vary in the degree of contact with humans. R. aegyptiacus roosts in caves but forages in orchards, whereas M. condylurus roosts in buildings. The results of this preliminary study suggest that some (2, 17, 26, 31) and -negative (38, 321) bat serum specimens tested using full-length recombinant SARS-CoV N and a fragment of the S protein (amino acids 318-510). Serum specimens were diluted 1:2,500 (left strips) and 1:5,000 (right strips). Secondary detection was performed by incubating the nitrocellulose strips with horseradish peroxidase (HRP)labeled goat-antibat immunoglobulin (Ig) (Bethyl, Montgomery, AL, USA) (1:10,000). For chemiluminescence, SuperSignal Dura substrate (Pierce Biotechnology, Rockford, IL, USA) was added and fi lms exposed for 1 min. Serum 17* was used as a reference for comparing blots. For evaluation purposes, strips were also incubated with human SARS-CoV-positive (A, B) and -negative serum specimens C and D (HCoV-NL63 positive) at the same dilutions, using goat-antihuman Ig HRP (1:20,000) for secondary detection. Serum specimens that produced signals at a dilution of 1:5,000 were recorded as positive (+). Vero E6 cells infected with severe acute respiratory syndromeassociated coronavirus (SARS-CoV). The SARS-CoV diagnostic IIFT kit (EUROIMMUN AG, Lübeck, Germany) was used with minor modifi cations: bat and reference human serum specimens were diluted 1:100 (found to be the optimal dilution for bat sera) in sample buffer, and secondary detection was performed with goat-antibat immunoglobulin (Ig) (Bethyl, Montgomery, AL, USA) followed by fl uorescein isothiocyanate (FITC)-labeled donkeyantigoat Ig (Dianova, Hamburg, Germany) (A-F) or FITC-labeled goat-antihuman Ig (G-I). Frames A-D, SARS-CoV ELISA-positive bat serum specimens 2, 17, 26, 31; E-F, ELISA-negative bat serum specimens 38 (showing unspecifi c signals) and 306; G-H, SARS-CoV-positive human control serum specimens A and B; I, negative human serum C. All photographs were taken at equivalent microscope settings. Scale bars represent 20 μm. of the African bat species harbor agents related to putative group 4 CoV, and therefore further investigations should be undertaken to determine potential public health risks. Coronavirus as a possible cause of severe acute respiratory syndrome Identifi cation of a novel coronavirus in patients with severe acute respiratory syndrome A novel coronavirus associated with severe acute respiratory syndrome Isolation and characterization of viruses related to the SARS coronavirus from animals in southern China Bats are natural reservoirs of SARS-like coronaviruses Severe acute respiratory syndrome coronavirus-like virus in Chinese horseshoe bats Prevalence and genetic diversity of coronaviruses in bats from China Bats: important reservoir hosts of emerging viruses Review of bats and SARS Human coronavirus NL63 employs the severe acute respiratory syndrome coronavirus receptor for cellular entry On-column protein refolding for crystallization Assessment of IgG antibodies against yellow fever virus after vaccination with 17D by different assays: neutralization test, haemagglutination inhibition test, immunofl uorescence assay and ELISA Generic detection of coronaviruses and differentiation at the prototype strain level by reverse transcription PCR and nonfl uorescent low-density microarray Evaluation of human monoclonal antibody 80R for immunoprophylaxis of severe acute respiratory syndrome by an animal study, epitope mapping, and analysis of spike variants We thank A. Teichmann for excellent technical assistance. We also thank Lia van der Hoek for providing us with HCoV-NL63-positive serum specimens.Mr Müller is a scientist at the Center for Biological Safety of the Robert Koch-Institut, Berlin. He has been involved in establishing diagnostic tools for SARS-CoV detection, assisted international quality assurance studies on SARS diagnostics, and worked on SARS-CoV susceptibility studies. Currently he is fi nishing his PhD thesis on expression analysis of coronavirus structural proteins.