key: cord-352768-16vgnq14 authors: Tang, Qingquan; Li, Baojian; Woodle, Martin; Lu, Patrick Y. title: Application of siRNA Against SARS in the Rhesus Macaque Model date: 2008 journal: RNAi DOI: 10.1007/978-1-59745-191-8_11 sha: doc_id: 352768 cord_uid: 16vgnq14 Containment of the SARS coronavirus (SCV) outbreak was accompanied by the rapid characterization of this new pathogen's genome sequence in 2003, encouraging the development of anti-SCV therapeutics using short interfering RNA (siRNA) inhibitors. A pair of siRNA duplexes identified as potent SCV inhibitors in vitro was evaluated for in vivo efficacy and safety in a rhesus macaque SARS model using intranasal administration with clinical viable delivery carrier in three dosing regimens. Observations of SCV-induced SARS-like symptoms, measurements of SCV RNA presence in the respiratory tract, microscopic inspections of lung histopathology, and immunohistochemistry sections from 21 tested macaques consistently demonstrated siRNA-mediated anti-SCV activity. The prophylactic and therapeutic efficacies resulted in relief of animals from SCV infection-induced fever, diminished SCV in upper airway and lung alveoli, and milder acute diffuse alveoli damage (DAD). The dosages of siRNA used, 10 to 40 mg/kg, did not show any sign of siRNA-induced toxicity. These results support that a clinical investigation of this anti-SARS siRNA therapeutic agent is warranted. The study also illustrates the capability of siRNA to enable a massive reduction in development time for novel targeted therapeutic agents. We detail a representative example of large-mammal siRNA use. The outbreak of severe acute respiratory syndrome (SARS) posed an urgent need to understand disease pathogenesis (1-3) and biology of the causative agent, now identified as SARS coronavirus (SCV) (4-8). SARS 139 develop a high fever followed by severe clinical symptoms including acute respiratory distress syndrome (ARDS) with diffuse alveolar damage (DAD) at autopsy (2, 4, 9) . The containment of SARS was achieved largely through traditional quarantine and sanitation measures (9,10). Since SARS is a newly emerging disease and the first coronavirus-mediated disease, a safe and effective vaccine was not available, nor was an established anti-coronavirus therapeutic (11) . Candidate vaccines became possible only once the causative virus was identified; efforts already have advanced to monkey models and clinical testing, spanning many approaches from attenuated and modified vaccinia virus, MVA (12), recombinant parainfluenza virus, BHPIV3 (13), inactivated whole virus (11), to DNA vaccines (14) . However, these rapid advances require rigorous and lengthy studies (15), illustrating the difficulty in using vaccine development to offer rapid solutions for new emerging infectious diseases. To treat SARS patients, combinations of existing drugs have been developed including ribavirin, antibiotics, anti-inflammatory steroids, and immune stimulators, and this approach had achieved some clinical successes ( [16] [17] [18] [19] [20] [21] . Many ongoing efforts to develop SARS-specific drugs such as screening of small molecule inhibitors and current biological approaches will clarify the strengths and weaknesses of each approach, based on the ultimate success rate, and the time and cost incurred. The identification of SCV as the causative pathogen of SARS was critical for containment and patient management. This was achieved mainly by demonstration that exposure of cynomolgus macaques to SCV resulted in similar symptoms to those of SARS patients (1,2) while also creating the first animal disease model critical not only for understanding SARS pathogenesis but also for evaluating potential vaccines and novel therapeutics (13) and was followed by the development of several others (12, 14, 17, 22) . Demonstration of protection by PEGylated interferon-from SCV infection in cynomolgus macaques, as seen in SARS patients, gives further proof of the effectiveness of such model (21) . Recently, a rhesus macaque model for SARS has been established with intranasal instillation of SCV strain PUMC01, showing many elements of pathology similar to those of SARS patients and the cynomologus macaque model (see Notes 1-3). The pathogeneses include elevated body temperature, low appetite, and acute DAD clearly visible at 7 days' post-infection (d.p.i.), but with somewhat worse severity (23-26). Thus, it offers an ideal model for evaluation of therapeutic candidates inhibiting SCV specifically as potential treatments for SARS. The search for developing antiviral agents directly from viral genome sequences has led to thorough investigations of siRNA (27, 28) . We previously screened 48 siRNA candidates targeting elements throughout the entire SCV genome and identified several active siRNA duplexes using fatal rhesus monkey kidney (FRhK-4) cells (29) . Other active siRNA sequences inhibiting SCV have also been reported from screening only a handful of candidate open reading frames in cell culture with either synthetic siRNA (30-32) or plasmidexpressed shRNA (33). Translation from in vitro inhibition to efficacious use to treat clinical respiratory infections depends on clinically acceptable and effective administration. A pair of siRNAs showing prominent prophylactic and therapeutic activities in the cell culture study (29), referred to as siSC2 and siSC5, were further evaluated in vivo, first in mice using a reporter gene assay and subsequently using a clinically acceptable intranasal administration in the recently established rhesus macaque SARS model (23-26). The study revealed strong evidence that these siRNA duplexes are potent prophylactic and therapeutic anti-SARS agents, and there is a lack of toxicity in the nonhuman primate model. These results further support the growing expectation that siRNA can fulfill the need for moving rapidly from gene sequence to selective inhibitory agents, and for many previously intractable therapeutic targets (see Notes 4 and 5). We offer representative examples of our procedures and the corresponding results. We expect that readers will test their own targets and optimize the protocol accordingly. 1. Two SCV-specific siRNA duplexes, siSC2 and siSC5, targeting, respectively, the SCV genome at spike protein and ORF1b (nsp12) coding regions, were designed based on SCV complete genome sequence (NC-004718), derived from strain TOR-2 (AY274119). 2. Selection of siSC2 and siSC5 was based on their anti-SARS potencies validated in the cell culture study (29); they were always used as a mixture (siSC2-5) of equal amounts. 3. A pair of control siRNA duplexes, siCONa and siCONb, without any homology to human and SARS genomes, were also used in the mixture (siCONa-b). Another pair of unrelated control siRNA duplexes, siCONc and siCONd, were used in the mixture in the mouse study (siCONc-d). 4. All siRNA duplexes consist of two complementary 21-nt RNA strands with 3 dTdT-overhangs and were manufactured by Qiagen (Gaithersburg, MD): siSC2: 5 -GCUCCUAAUUACACUCAACdtdt-3 3 -dtdtCGAGGAUUAAUGUGAGUUG-5 siSC5: 5 -GGAUGAGGAAGGCAAUUUAdtdt- 3 3 -dtdtCCUACUCCUUCCGUUAAAU-5 siCONa: 5 -CCGCUGGAGAGCAACUGCAdtdt- 3 3 -dtdtGGCGUCCUCUCGUUGACGU-5 siCONb: 5 -GCUAUGAAACGAUAUGGGCdtdt- 3 3 -dtdtCGAUACUUUGCUAUACCCG-5 siCONc: 5 -GCUGACCCUGAAGUUCAUCdtdt- 3 3 -dtdtCGACUGGGACUUCAAGUAG-5 siCONd: 5 -GCAGCACGACUUCUUCAAGdtdt-3 3 -dtdtCGUCGUGCUGAAGAAGUUC-5 For cost-saving purposes and to minimize handling of the pathogenic SCV, the mouse is first used to screen a large number of siRNAs against recombinant SCV targets before moving to the monkey. 1 . Divide 20 BALB/c mice (6-8 weeks old) into four groups (N = 5). 2. The pCI-scLuc reporter plasmid was constructed earlier by inserting a DNA fragment containing siSC2 and siSC5 targeted sequence DNA between its CMVdriven transcriptional initiation site and luciferase coding sequence. 3. Two carrier solutions, D5W and Infasurf TM (see Note 6), were used for intratracheal deliveries of the siSC2-5, siCONc-d, and pCI-scLuc plasmids. A typical example of study design is shown in Table 1 (see Notes 8-12). 1. Inoculate SCV-negative healthy monkeys with PUMC01 at 10 5 TCID50/1.0 mL through nasal instillation, mimicking the natural route of SCV infection of SARS patients. 2. Also deliver 30 μg of siSC2-5 and siCONa-b siRNA agents in 3 mL of D5W intranasally. 3. After the macaques are SCV-challenged and treated with siSC2-5 or siCONa-b, observe for clinical signs daily, including body temperature, size of lymph nodes, body weight, coughing, sneezing, appetite, aggressiveness, etc. including liver enzymatic analysis and the SARS-specific antibody detection as detailed below. 6. For liver enzymatic analysis, we chose alanine aminotransferase (ALT), lactic acid dehydrogenase (LDH), creatine kinase (CK), and aspartate aminotransferase (AST) at 7 d.p.i. after the SCV infection of all 20 animals from every tested group. Their levels should all increase. In our experiments, routine blood examination also indicated a marked increase of hemoglobin (HGB) and platelets (PLT) in SCV-infected macaque, which is contradictory to another report on the macaque SARS model (22) and reports on SARS patient (9,10,16). 7. Detect anti-SCV IgG or IgM by standard ELISA. 8. When the macaques are necropsied at 7 and 20 d.p.i., collect lungs and conduct thorough microscopic inspections of lung histopathology. 9. Collect other organs as needed with appearance and morphology inspections and further compare using an internal organ coefficient of each group, based on wet weight of organ per 100 g of average body weight. 1. Isolate total cellular RNA using a QIAamp RNA isolation kit (Qiagen). Synthesize the first strand of cDNA using RNAse H + reverse transcriptase and random primers (Invitrogen), according to manufacturer's protocol. The forward and reverse primers and the fluorescence probe used for PCR were 5 -GCATGAAATTGCCTGGTTCAC-3 , 5 -GCATTCCCCTTTGAAAGTGTC-3 , and FAMAGCTACGAGCACCAGACACCCTTCGAAATRMA, respectively. 2. Perform real-time PCR using ABI7900 Sequence Detection System (ABI, CT) and all PCR in triplicates. 3. Perform SCV reisolation using the swab samples by serial passage on Vero cell culture as previously described (24,25). 1. Create epoxy resin-filled lung blocks from the right upper and right middle lobes and perform routine pathology analysis. Briefly, first fix the tissues with 10% formaldehyde, embed in resin, section, stain with H&E or silver stain, and then subject to microscopic examination. 2. The severity of lung damage is determined based on observations of five different sections of each lung by readouts from three independent pathologists with blind sample IDs. 3. Resin-embedded tissue sections are "de-waxed" and rehydrated for the immunohistochemistry analysis as follows. Incubate the tissue sections in 0.3% hydrogen peroxide for 30 min and rinse with PBS. Then treat with normal sera in humid chamber for 20 min, and treat with a 1:100 diluted primary antibody followed by a treatment with appropriate 1:1,000 diluted secondary antibody. 4. After substrate staining and hematoxylin counterstaining, examine the slides under microscope. Our first antibody was the convalescent antisera from a SARS patient of PUMH (STS-D, Zhang-03), and the second antibody was a biotinylated goatanti-human IgG (PK-4001, ABC kit). 5. Identify the cell types based on the separate staining with corresponding mAbs using methods described previously (24,25) . 6 . The SCV-infected cell counts within each microscopic image from every lung tissue section are independently collected by three readouts with blind sample IDs. Average cell counts of four lungs from each group (N = 4) are compared. 1. We analyzed data using the Student t-test for Luciferase expression in mouse lungs (Fig. 1d) , mean body temperature (Fig. 4a) , histopathology score comparison (Fig. 4d) , and SCV-infected cell counts (Fig. 5h ). 2. Statistical significance is only considered when P < 0.05. The regression analysis is conducted based on the average body temperature of each group at each day point (Fig. 4b) . 1. While concern remains whether the macaque SARS models have good clinical relevance (15, [22] [23] [24] [25] [26] , the rhesus macaque model in the present study using a highly virulent SCV strain PUMC01 simulates the pathogenesis process in SARS patients (9,10,39). Clear clinical relevance of this model is found in most of the parameters studied including elevated body temperature, lung pathology, and SCV antigen detection in epithelial originated type I pneumocytes, type II pneumocytes, and macrophages, providing strong support that the model has the attributes required for evaluation of anti-SCV siRNA. 2. In this study the siSC2-5 was dosed through the same intranasal route as the SCV challenge, with prophylactic, concurrent, or early postexposure treatments within a period of 5 d.p.i. All three different treatment regimens achieved potent suppression of SCV-induced SARS pathogenesis. Detection of the SCV RNA genome with RT-PCR revealed that only 25% of oropharyngeal swab samples from the treated group were positive versus all samples from the control groups being positive. Similarly, using immunohistochemistry detection, SCV-infected cell counts significantly decreased in the lung sections from the treated groups. Along with the reduced viral spread was a substantial reduction in the SARS-like clinical symptoms and the lung histopathology. 3. A few comments regarding the mechanism of siRNA action against SCV are in order. The present study is designed to investigate the siRNA-mediated anti-SCV effects in both the upper airway and deep lung of SCV-exposed macaques that occurred during the early phase of the viral infection and disease progression. The impact of the siSC2-5 on the early phase of SCV infection is first exhibited in the mucosal epithelial cells of the upper respiratory tract, expected since siSC2-5 and SCV are both administered through intranasal instillation and all siRNA dosings are completed within the first 5 days. This siSC2-5 anti-SARS efficacy can result from one or more of the following three possible mechanisms: protection of cells from a successful SCV infection; degradation of SCV mRNA inhibiting viral protein synthesis in infected cells (29); or obstruction of SCV genome replication and spread to uninfected cells. Here a single prophylactic dose of siSC2-5 provides protection comparable to therapeutic treatment using multiple doses. Similar clinical benefits were observed from both treatment regimens of CD and PE, indicating that researchers may try to improve dosages and regimens. These studies with an early siRNA intervention in SCV exposure resulted in a long-lasting inhibitory effects on the average body temperature, viral infected cell counts, and lung damage for 20 days. Considering that SARSspecific neutralizing antibody in SCV-infected macaques can be detected as early as 10 d.p.i., we speculated that the clinical benefit of siRNA-mediated anti-SARS activity observed in this study is the consequence of combined activities from the siRNA agent and the neutralizing antibody, suggesting that multiple antiviral mechanisms were operative (also see Note 12). 4. There are interesting advantages to using siRNA in SARS (29,34) . The release of proinflammatory cytokines from the alveolar macrophage has been proposed to play a prominent role in SARS pathogenesis and as a point for intervention ( In contrast to such proinflammatory cytokine treatments, intranasal delivery of siRNA offers a unique compliment of high-specificity inhibition of the target SCV with minimal induction of a proinflammatory cytokine antiviral response that may help to avoid exacerbating symptoms and lung damage. Reports of siRNA administration in mouse models for lung delivery have evaluated different formulations including cationic polymer and lipid complexes using either intravenous or airway administration (34-37) and shown efficient anti-RSV and anti-influenza effects as well (e.g., see Chapter 6). 5. Selection of potent SCV-specific siRNA agents: Two siRNA duplexes, siSC2 and siSC5, targeting the SCV genome at spike protein coding and ORF1b (nsp12) regions, respectively, were chosen for in vivo studies for the following reasons: (a) The targeted sequences of these two siRNA duplexes exhibit a 100% homology to the strain TOR-2 used in the cell culture study (29) , to the strain PUMC01 used in the macaques model, and to the more than 100 other published SCV strains, representing those isolated during different phases of the SCV evolution as recently defined (6) with wide geographic distributions around the world (Fig. 1a) ; (b) siSC2 and siSC5 are the two most potent inhibitors for reducing SCV replication in FRhK-4 cells, among a set of active siRNA duplexes selected from 48 siRNA duplexes targeting entire SCV genome (29); (c) a synergic effect of anti-SCV activity was observed when a combination of siSC2 and siSC5 was applied in the cell culture study, showing the strongest prophylactic and therapeutic effects (Fig. 1b, c) among many other combinations with those active siRNA duplexes (29); (d) the targeted sequences of siSC2 and siSC5 share no homology to the human genome, avoiding potential nonspecific knockdown of patient endogenous genes. In addition, a pair of nonrelated siRNA duplexes, siCONa and siCONb, with no homology to either the human genome or the SARS genome, validated in the cell culture study showing no RNAi activity for SCV inhibition, was chosen as the negative control in the macaque study. 6. Carrier/delivery reagent: TransIT-TKO and polyethyleneimine (PEI) have been reported as carriers for intranasal (35), intratracheal (36), and intravenous (37) deliveries of siRNA into mouse models for treatments of influenza virus and RSV infections. However, these carriers are not feasible for clinical use; PEI, in particular, can induce severe lung inflammation through either intravenous and intratracheal delivery in mice based on our experience and the literature (35,37-40) . We have tested D5W solution (41) and Infasurf ™ solution (42), which were also applied in animal model deliveries of DNA (43) and siRNA (44). Codelivery of pCI-scLuc plasmid with siSC2-5 in D5W solution illustrates a higher level of reporter gene expression and stronger RNAi effect than those in the Infasurf ™ solution (Fig. 1d) . 7. Amount of nucleic acid: We have observed no lung damage with intratracheal delivery of 60 μg of the nucleic acid, providing a safe baseline for siRNA dosing in the respiratory tract of larger mammals. 8. Scoring of pathology in rhesus macaques: Varying degrees of severity of lung damage are scored in microscopic inspection of tissue sections. We adopted a six-grade scoring system (Fig. 2a-f) : (1) "normal," lung tissue from the control animal without SCV infection; (2) "±", almost normal, slightly broadening of alveolar septa and sparse monocyte infiltration; (3) "+", hemorrhage in septa, elastic fibers of alveolar wall distorted as shown by silver staining; (4) "++", alveolus septa broadening with increasing infiltration of inflammatory cells; (5) "+++", extensive exudation and septa broadening, shrinking of alveoli caused by pressure, restricted fusion of the thick septa, obvious septa hemorrhage, ruptured elastic fiber of alveolar wall, and slight filtration in alveolar cavities; (6) "++++", massive cell filtration and alveoli shrinking, sheets of septa fusion, necrotic lesions at the hemorrhagic septa, and massive cell filtration in alveolar cavities. 9. Features of acute DAD in SCV-infected rhesus macaque lungs: SCV-induced DAD in lower airway was first observed in SARS patients with disease for more than 10 days (9), while the SCV-infected macaque lungs started developing acute . (21,23) . In histopathology and immunohistochemistry microscopic inspection, we found that most of the necropsied lungs had developed acute DAD with various degrees of severity. The typical features of the SCV infection-induced lung (both 7 and 20 d.p.i.) are (a) broken alveolar walls and interstitial edema (Fig. 3a) ; (b) hyaline-membrane formation along the alveoli and pneumocyte desquamation (Fig. 3b) ; (c) damaged alveolus filled with hemorrhage and pneumocytes with nuclear enlargement, prominent nucleolus, and amphophilic granular cytoplasm (Fig. 3c) ; and (d) interstitial infiltrates with neutrophils, lymphocytes and macrophages (Fig. 3d) . Within damaged lung tissues, one can also identify viral-infected pneumocytes, infiltrated neutrophils, lymphocytes, and monocytes that are characteristic of lung inflammation and characterized using keratin (Fig. 3e) , CD68 (Fig. 3f) , CD4, CD8, and CD35 immunohistochemical staining (data not shown). These observations are very similar to the lung damage observed in human patients (9,10) and in a couple of the SARS macaque models (21-23) . 10 . Suppression of SARS-like symptoms by siRNA: An effective siRNA will reduce essentially all clinical symptoms described above, showing significant lowering shows the alveolar walls collapsed and acute diffuse interstitial injury with interstitial edema as arrows indicated at early stage of the disease; (b) section from macaque #015 shows hyaline-membrane formation indicated with arrows along the alveoli and pneumocyte desquamation. (c, d) Lung sections stained with H&E at high-power magnification of X200: (c) Section from macaque #166 shows damaged alveoli were filled with hemorrhage and inflammatory cells indicated by arrows and pneumocytes with nuclear enlargement, prominent nucleolus and amphophilic granular cytoplasm resulting in focal giant-cell formation as arrows indicate; (d) section from macaque #202 shows the inflammatory cells, including neutrophils, lymphocytes, macrophages, and monocytes, were presented in the damaged alveoli. (e) IHC staining of SCVinfected monkey lung section with keratin-specific mAb indicates the epithelium origin pneumocytes pointed to by arrows, X200. (f) IHC staining of SCV-infected monkey lung section with CD68 mAb indicates microphage infiltrates as arrow points, X400. of pathology scores. Suppression of SCV-induced fever is one of the most obvious and easily detectable siRNA effects in the rhesus macaque model. SCVspecific IgG titer in every blood sample collected at various time points also illustrates an inhibitory effect of siSC2-5 in treated animals (Fig. 4c) . The SCVspecific IgG levels in IC and NS groups are detected as early as 10 d.p.i., but not in the CD and PE groups. Interestingly, the SCV specific IgG of PL group is detected at 10 d.p.i., suggesting a different mechanism of action for anti-SARS activity. Meanwhile, the SCV-specific IgG levels of all groups are well above detectable level at 19 d.p.i. 11. Inhibition of SCV replication in macaque respiratory tract by siRNA: In addition to acting as an antiviral in the lung, the siRNA shows strong efficacy in the upper respiratory tract. This can be revealed by RT-PCR analysis of oropharyngeal swab samples at 4 d.p.i. (Fig. 5) . 12. Prophylactic effects of siRNA: Note that delivering the siSC2-5 prior to SCV infection in PL group using a single dose is able to achieve a comparable inhibitory effect to that of the CD and PE groups. This prophylactic anti-SCV activity resulted in lowered body temperature (Fig. 4a, b) , milder lung damage (Fig. 4d) , less viral RNA detected (Fig. 5a) , and lowered numbers of SCVinfected cells in the lung (Fig. 5h) , in comparison with the CD and PE treatment groups. This prophylactic efficacy could be a combination of direct degradation of viral RNA by pre-existing intracellular siSC2-5 within the upper airway cells when the viral particle enters, decreasing replication and spread of SCV particles reaching deeper into the lungs, and a cellular antiviral activity induced by siRNA transfection (other than interferon response, (45-53) ). 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