Effect of Antiflagellar Human Monoclonal Antibody on Gut-Derived Pseudomonas aeruginosa Sepsis in Mice

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Clinical and Diagnostic Laboratory Immunology, July 1999, p. 537-541, Vol. 6, No. 4
1071-412X/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.

Effect of Antiflagellar Human Monoclonal Antibody on Gut-Derived Pseudomonas aeruginosa Sepsis in Mice

Tetsuya Matsumoto,¹^,^* Kazuhiro Tateda,¹ Shuichi Miyazaki,¹ Nobuhiko Furuya,¹ Akira Ohno,¹ Yoshikazu Ishii,¹ Yoichi Hirakata,² and Keizo Yamaguchi¹

Department of Microbiology, Toho University School of Medicine, Omori-Nishi, Ota-ku, Tokyo,¹ and Department of Laboratory Medicine, Nagasaki University School of Medicine, Sakamoto, Nagasaki,² Japan

Received 31 August 1998/Returned for modification 19 January 1999/Accepted 23 April 1999

	ABSTRACT

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We evaluated the effect of antiflagellar human monoclonal antibody on gut-derived Pseudomonas aeruginosa sepsis. Mice weregiven a suspension of P. aeruginosa SP10052 in their drinkingwater and were simultaneously treated with ampicillin (200 mg/kgof body weight) to disrupt the normal bacterial flora. Cyclophosphamidewas then administered to induce leukopenia and translocation ofthe P. aeruginosa that had colonized the gastrointestinal tract,thereby producing gut-derived generalized sepsis. In this model,intraperitoneal injection of 100 µg of antiflagellar human monoclonalantibody (SC-1225) per mouse for 5 consecutive days significantly(P < 0.01) increased the survival rate compared with that formice treated with bovine serum albumin (BSA). Treatment with SC-1225significantly reduced the average number of viable bacteria inportal blood, liver, and heart blood compared with the averagenumber after treatment with BSA. Furthermore, the presence inserum of the inflammatory cytokines tumor necrosis factor alphaand interleukin 6 were evaluated as markers of severity of infection,and the results showed that the levels of these cytokines in micetreated with SC-1225 were significantly decreased in comparisonwith those in BSA-treated control mice. Although there was nosignificant difference in the number of bacteria that colonizedthe intestine, SC-1225 treatment significantly increased bacterialopsonophagocytosis by cultured peritoneal macrophages from micewith or without cyclophosphamide pretreatment. Our results indicatethat antiflagellar human monoclonal antibody SC-1225 protectsmice against gut-derived sepsis caused by P. aeruginosa and suggestthat such an effect is due to its opsonophagocytic activity andthe reduced motility of the translocated bacteria once the bacteriamove from the intestine into thebloodstream.

	INTRODUCTION

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Infection with Pseudomonas aeruginosa, a common pathogen that causes septicemia in immunocompromised hosts, has a higher fatalityrate than any other gram-negative bacterial infection. Althoughantibiotic therapy is thought to be the most effective therapyagainst infections caused by this microorganism, such therapyis frequently ineffective due to bacterial resistance. Therefore,effective immunotherapy may be a useful alternative therapy administeredeither alone or in combination with antibioticchemotherapy.

Some reports have shown that neutrophils (36), complement (2), and immunoglobulins (32) play important roles in hostdefense against P. aeruginosa infection. However, P. aeruginosais frequently identified as a causative agent of sepsis in immunocompromisedpatients with neutropenia induced by antineoplastic chemotherapy(13). Because normal neutrophil function is not expected inpatients with neutropenia, humoral immune responses may play amore important role in the recovery of such patients from P. aeruginosainfection. Vaccination with microbial antigens may be the mosteffective method for the induction of protective humoral immuneresponses (9). However, vaccination of immunocompromised hostsis frequently unsuccessful due to immunodeficiency (18). Therefore,passive immunization may be a more practical method for immunotherapyto protect individuals against P. aeruginosainfection.

Because experimental data suggest that lipopolysaccharide (LPS) is an important virulence factor in P. aeruginosa infection,the protective action of anti-LPS antibody or polysaccharide vaccineshas attracted the attention of several groups of investigators(8-10, 34, 35). Unfortunately, however, due to the presenceof various LPS serotypes of P. aeruginosa, it is difficult toproduce protective antibodies against a broad spectrum of P. aeruginosaisolates (10, 30, 34, 35, 38, 40). In contrast toLPS, there are only two known serotypes (designated serotypesa and b) of P. aeruginosa flagella (5). Flagella are also importantvirulence factors in P. aeruginosa infection (14, 17). Thus,antibodies against flagellar antigens may be more useful thanthose directed against LPS in protecting hosts against a widerange of P. aeruginosa infections. These considerations led usto investigate the effects of antiflagellar antibodies on murinegut-derived P. aeruginosa sepsis associated with neutropenia inducedby antineoplasticchemotherapy.

	MATERIALS AND METHODS

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MAb. Human immunoglobulin M (IgM) monoclonal antibody (MAb) SC-1225 was kindly provided by Sumitomo Pharmaceuticals Co., Osaka,Japan. This MAb, which specifically reacts with b-serotype flagella,is purifiedchromatographically.

Bacterial strain. P. aeruginosa SP10052, a clinical isolate that is known to react with MAb SC-1225 (39), was also provided by Sumitomo Pharmaceuticals.The strain was kept frozen at $-$ 80°C in Mueller-Hinton broth (DifcoLaboratories, Detroit, Mich.) containing 15%glycerol.

Animals. Inbred, specific-pathogen-free male ddY mice (Japan Shizuoka Laboratory Center Co., Shizuoka, Japan) weighing 20 to 24 g wereused in our experiments. The animals were housed in sterile cagesand received sterile distilled water except when P. aeruginosawas being orally administered. The experimental protocol was approvedby the Institutional Animal Care and Use Committee at Toho UniversitySchool ofMedicine.

Survival of mice with gut-derived P. aeruginosa sepsis. Gut-derived P. aeruginosa sepsis was produced as described previously (24, 26). Briefly, bacteria were grown on Trypticasesoy agar (BBL Microbiology Systems, Cockeysville, Md.) at 37°Cfor 18 h, suspended in sterile 0.45% saline, and adjusted to aconcentration of 10⁷ CFU/ml. The bacterial suspension was added to the drinking wateron days 1 to 3. To promote colonization of P. aeruginosa SP10052,which is insensitive to ampicillin (ABPC), 200 mg of ABPC perkg of body weight was administered by daily intraperitoneal injectionson days 1 to 3 in order to produce a disturbance of the normalintestinal flora. This was followed by intraperitoneal injectionof 150 to 200 mg of cyclophosphamide per kg on days 5 and 8. Eachexperiment was repeated at least twice. The lethal effects ofinfection were checked every 24 h for 7 days (see Fig. 1). MAbSC-1225 was injected intraperitoneally (100 µg/day) for 5 days,commencing after administration of the second cyclophosphamidedose. Control mice received identical amounts of bovine serumalbumin(BSA).

Tissue sampling and determination of viable bacteria. Mice from each treatment group were killed by exposure to ether at the indicated time intervals. Under aseptic conditions,blood samples were taken from the portal vein and cardiac chamber.Under similar conditions, liver tissue specimens were obtainedand were immediately homogenized in sterile saline. Portions ofthe blood samples and liver homogenates were plated onto Trypticasesoy agar and were cultured at 37°C for 24 h to detect and identifythe P. aeruginosa challenge strain. The remaining blood sampleswere allowed to clot at 4°C in sterile glass tubes and were thencentrifuged at 2,000 × g for 15 min. Serum samples were preservedat $-$ 80°C until measurement of cytokinelevels.

Determination of intestinal colonization. Fecal samples were collected from mice 4 days after administration of the second dose of cyclophosphamide. The samples wereweighed and were homogenized with 2 ml of sterile saline, andthe homogenates were serially diluted. Fifty-microliter portionsof the various dilutions were plated onto NAC agar (Eiken ChemicalCo., Tokyo, Japan) and were cultured at 37°C for 24 h. The numberof CFU per gram was calculated by counting the number of coloniesthat grow on theagar.

Opsonophagocytosis of bacteria by cultured murine macrophages. The effect of MAb SC-1225 on phagocytosis of P. aeruginosa SP10052 by murine peritoneal macrophages was assessed as follows.Peritoneal macrophages freshly drawn from untreated healthy micewere washed twice with RPMI 1640 medium (Nissui PharmaceuticalCo., Tokyo, Japan), after which 500 µl of the resulting cell suspension(10⁶ cells/ml) was placed into each well of a 24-well tissue cultureplate (Falcon 3047; Becton Dickinson & Co., Franklin Lakes, N.J.)and the plate was incubated for 1 h. Bacteria at the logarithmicgrowth phase was suspended with RPMI 1640 medium at a concentrationof 10⁵ CFU/ml and were incubated for 30 min without or with 0.1 or 1µg of SC-1225 per ml. Five hundred-microliter volumes of eachbacterial suspension were added to separate wells of a tissueculture plate, and the mixture was incubated with rocking for2 h at 37°C in 5% CO₂. The number of viable bacteria in the culturesupernatants was determined by plating the supernatant on Mueller-Hintonagar and culturing at 37°C for 24h.

Furthermore, we determined the effects of MAb SC-1225 on phagocytosis by using peritoneal macrophages from mice treated with200 mg of cyclophosphamide per kg intraperitoneally 1 or 2 daysbefore theassay.

Cytokine assay. Tumor necrosis factor alpha (TNF- $alpha$ ) and interleukin 6 (IL-6) levels in mouse serum were determined with enzyme-linked immunosorbentassay (ELISA) kits (Endogen Inc., Boston, Mass.). IL-1 $beta$ concentrationswere assessed with a commercially available ELISA kit (GenzymeCorp., Boston, Mass.). The assays were performed exactly as describedby the manufacturers, and the levels in each sample were determinedinduplicate.

Statistical analysis. Differences in survival rates among groups were evaluated by the chi-square test. Viable bacterial counts and cytokine concentrationswere compared by the Mann-Whitney U test. A P value of $<=$ 0.05 wasconsideredsignificant.

	RESULTS

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Effect of antiflagellar MAb on survival of mice. We measured the protective effect of an antiflagellar MAb (MAb SC-1225) in mice with gut-derived P. aeruginosa sepsis. Asshown in Fig. 1, the survival rate of mice treated with SC-1225was significantly higher than that of the control mice (P < 0.01).These results suggest that administration of SC-1225 protectsmice against gut-derived sepsis.

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FIG. 1. Effect of antiflagellar MAb on the survival of mice with gut-derived P. aeruginosa sepsis. Each mouse (n = 10) received 100 µg of an antiflagellar human MAb (MAb SC-1225) for 5 consecutive days at 24-h intervals following the second cyclophosphamide treatment by intraperitoneal injections. Control mice (n = 10) received 100 µg of BSA on the same schedule. CY, cyclophosphamide.

Effect of antiflagellar MAb on viable bacterial counts. In our mouse model, P. aeruginosa isolates that colonize the gastrointestinal tract invade the bloodstream and, after breakingthrough the defense system provided by the liver, spread intothe systemic circulation. We therefore examined viable bacterialcounts in the portal blood, liver, and heart blood in mice treatedwith antiflagellar MAb and in control BSA-treated mice. The resultsdemonstrated that administration of SC-1225 significantly suppressedthe number of viable bacteria in the portal blood, liver, andheart blood (Table 1).

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TABLE 1. Effect of antiflagellar MAb on the number of viable bacteria in various organs^a

Influence of antiflagellar MAb on serum cytokine levels during gut-derived sepsis. Since the inflammatory cytokines TNF- $alpha$ , IL-1 $beta$ , and IL-6 are thought to be good markers of the severity of bacterial infections(11, 24, 31), we determined the levels of these cytokinesin mice with gut-derived sepsis after antiflagellar MAb treatment.As depicted in Fig. 2, the results demonstrated significant decreasesin TNF- $alpha$ and IL-6 levels in SC-1225-treated mice in comparisonwith those in BSA-treated control mice. Although there was nosignificant difference, IL-1 $beta$ levels also showed a tendency todecrease in mice treated with SC-1225.

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FIG. 2. Influence of antiflagellar MAb on serum cytokine levels during gut-derived sepsis. MAb SC-1225 was administered intraperitoneally at 100 µg/mouse (closed columns) for 3 consecutive days at 24-h intervals following the second cyclophosphamide treatment. BSA was administered to control animals (open columns) at the same intervals. Serum samples were collected 3 days after administration of the second dose of cyclophosphamide. Values are means ± standard errors of the means (six mice in each group). Symbols: #, P < 0.05; §, P < 0.01.

Effect of antiflagellar MAb on colonization of P. aeruginosa in intestinal tract. Because the reservoir of P. aeruginosa in the model used in this study is thought to be the gastrointestinal tract, we determinedthe effect of MAb SC-1225 on the ability of the bacteria to colonizethe intestine. This was performed by measurement of viable bacterialcounts in the feces 4 days after administration of the seconddose of cyclophosphamide. The average numbers of viable P. aeruginosain the feces of SC-1225-treated mice and BSA-treated mice were7.2 × 10⁴ ± 2.8 × 10⁴ and 1.3 × 10⁵ ± 2.6 × 10⁴ CFU/g, respectively (means ± standard errors of the means). Althoughthe bacterial count in mice treated with SC-1225 was slightlylower than that in BSA-treated mice, the difference was notsignificant.

Influence of antiflagellar MAb on opsonophagocytosis. To evaluate another mechanism by which MAb SC-1225 might protect mice against gut-derived sepsis, we studied the effect ofthe antibody on in vitro opsonophagocytosis of P. aeruginosa SP-10052by murine peritoneal macrophages. The results are depicted inFig. 3A. Although incubation with 0.05 µg of SC-1225 per ml tendedto reduce the number of viable bacteria in the medium, the differencewas not statistically significant compared with the number foruntreated controls. However, incubation with 0.5 µg of SC-1225per ml significantly reduced the number of viable bacteria inthe medium compared with that for the untreated controls.

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FIG. 3. Effect of antiflagellar MAb on opsonophagocytosis of P. aeruginosa by murine peritoneal macrophages. P. aeruginosa SP10052 was preincubated with MAb SC-1225 and was then incubated with rocking in a 24-well tissue culture plate with peritoneal macrophages. (A) Counts of viable bacteria were determine in the culture supernatants of SC-1225-treated groups (final concentrations, 0.05 and 0.5 µg/ml) and a control group not treated with SC-1225. (B) Mice were treated with 200 mg of cyclophosphamide per kg intraperitoneally 1 or 2 days before the opsonophagocytosis test. Counts of viable bacteria were determined in the culture supernatants after incubation with peritoneal macrophages from mice treated with cyclophosphamide 1 or 2 days before the assay and incubated with 0.5 µg of SC-1225 per ml. For the control group, peritoneal macrophages were drawn from mice treated with cyclophosphamide 1 day before the assay and incubated without SC-1225. Each bar shows the average number of viable bacteria as a percentage of that in the untreated control group. CY, day of cyclophosphamide treatment; Ab, antibody concentration (in micrograms per milliliter). Data represent the means ± standard errors of the means (n = 8 for each group). Symbols: §, P < 0.01; #, P < 0.05 compared with the control group.

Because all in vivo experiments were performed with the cyclophosphamide-treated mice, we further evaluated the effects of0.5 µg of SC-1225 per ml on phagocytosis of P. aeruginosa by usingperitoneal macrophages from mice treated with cyclophosphamide1 or 2 days before the assay. The results revealed that SC-1225significantly reduced the number of viable bacteria in the mediumcompared with that for the control group even in a test with macrophagesfrom cyclophosphamide-treated mice (Fig. 3B). These results suggestthat the protective effects of SC-1225 might be mediated at leastin part by enhancement of opsonophagocyticactivity.

	DISCUSSION

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Clinical studies with surveillance cultures of fecal samples from immunocompromised patients suggest that the gastrointestinaltract may be a primary reservoir for opportunistic bacteria (37).Previous studies have shown that bacteria within the gut can crossthe gastrointestinal mucosal barrier and spread systemically,a process termed bacterial translocation (6, 12). Berg etal. (7) reported that gram-negative enteric bacilli of thegastrointestinal tract systemically translocate in mice treatedwith a combination of antibiotics and immunosuppressive drugs,such as penicillin G sodium and cyclophosphamide. We induced acuteenteritis by administering APBC and cyclophosphamide to specific-pathogen-freemice fed P. aeruginosa. In this model, P. aeruginosa colonizesthe intestinal tract and can invade body tissues after inductionof immunosuppression or disruption of the intestinal mucosal barrierby administration of cyclophosphamide. Once the bacteria escapeKupffer cells in the liver, they disseminate systemically, causingbacteremia and septicemia, which is usually followed by deathof the animal. This model therefore resembles the septicemia inhumans caused by pathogens derived from the intestinal tract,particularly in immunocompromised hosts (20).

Concerning the role of administration of cyclophosphamide in this model, we think that the effect of this compound on thenumber of neutrophils is important for the induction of sepsis.In our preliminary experiment, the leukocyte count decreased lessthan 1,000/mm³ for 3 to 4 days after cyclophosphamide treatment. Furthermore,we also determined that the activity of Kupffer cells is alsodepressed by the administration of cyclophosphamide (data notshown).

Our murine gut-derived P. aeruginosa sepsis model is suitable for studying the effects of antiflagella antibodies againstsepsis. We have previously used this model to evaluate the protectiveefficacy of immunization with heat-killed P. aeruginosa and foundthat such immunization provided complete protection against death(25). We also evaluated the protective efficacies of vaccinesprepared from P. aeruginosa alkaline protease, elastase, and exotoxinA toxoids. The results showed that a combination of alkaline proteaseand exotoxin A toxoids is a logical candidate as a vaccine againstP. aeruginosa sepsis (23). These studies established the efficacyof immunotherapy with antibodies in P. aeruginosasepsis.

The major finding of the present study was the protective effect of MAb SC-1225, an antiflagellar human MAb, against P. aeruginosasepsis. Our results also indicated that flagella are importantcomponents in the pathogenesis of gut-derived sepsis. The modelused in the present study incorporates four features: oral inoculationof bacteria, subsequent bacterial colonization, overgrowth inthe intestinal tract, and invasion into the bloodstream. Therefore,to determine the mechanism of action of SC-1225, we first investigatedthe number of viable bacteria in the portal blood, liver, andheart blood and found that they were significantly decreased bySC-1225. However, our results suggested that SC-1225 failed toinfluence intestinal colonization of the bacteria; the numberof P. aeruginosa isolates in the intestines of mice treated withSC-1225 was not lower than the number in control mice. These resultssuggest that administration of antiflagellar MAb reduced the motilityof translocated bacteria once the bacteria moved from the gastrointestinaltract into the bloodstream and then contributed to theprotection.

A number of studies have demonstrated the protective effects of antiflagellar antiserum or MAbs against lethal P. aeruginosainfections in a burn wound model (15, 19, 21, 28, 33,39) and in a pneumonia model (22, 29). Landsperger et al.(22) demonstrated that decreased bacterial motility by antiflagellarantibody is associated with a decreased pathogenicity of P. aeruginosain rat model of pneumonia (22). As a mechanism of protectiveeffects of antiflagellar antibodies, Anderson and Montie (3,4) reported that antiflagellar antibodies stimulate opsonophagocytosisof P. aeruginosa by polymorphonuclear leukocytes. The presentresults also showed that incubation with a high dose of MAb SC-1225accelerated opsonophagocytosis of P. aeruginosa. These findingssuggest that the opsonophagocytic activity of antiflagella antibodiesmay be another mechanism by which they exert their protectiveeffects against sepsis, besides their inhibitory activity on bacterialmotility. We also speculated that the other mechanism of the protectiveeffect of SC-1225 against gut-derived sepsis is the lesseningof bacterial translocation, and we are now investigating thispossibility.

Isolation and characterization of MAb SC-1225 (originally designated IN-2A8) was reported by Ochi et al. (28), who demonstratedthat it strongly inhibited bacterial motility in vitro. Uezumiet al. (39), however, reported that SC-1225 alone did not protectmice against intraperitoneal infection, while combination therapywith SC-1225 and imipenem-cilastatin significantly improved thesurvival rate. In the present study, we demonstrated a protectiveeffect for SC-1225 against murine sepsis without the simultaneoususe of antibiotics. We speculate that the reason for differentresults may be due to differences in the experimental design.For example, Uezumi et al. (39) inoculated the bacteria intraperitoneallyinto healthy mice, while we selected the oral route and used cyclophosphamide-treatedleukopenic mice. Furthermore, the model used by Uezumi et al.(39) represents acute sepsis; the rapid growth of the infectingbacteria, observed in both the peritoneum and blood, results inthe death of all mice within 10 h following infection. In ourmodel, however, few untreated mice were still alive on the 3rdor 4th day. Most significantly, however, our approach providesa specific model of gut-derived septicemia, in which bacterialtranslocation across the gut wall is a key step. This step isbypassed in the experimental model of Uezumi et al. (39).

A high dose of 10 µg of antiflagellar MAb was previously found to provide protection against P. aeruginosa pneumonia in theneutropenic mouse (29). Uezumi et al. (39) initially usedthat dose; however, it was found to be ineffective in their model,and a higher dose, e.g., 100 or 500 µg per mouse, was needed.Similarly, our preliminary experiments showed that a dose of 10µg of MAb SC-1225 per mouse was ineffective against gut-derivedsepsis in the model used in the present study (data not shown).The protective effect of this MAb was noted only when the dosewas increased to 100 µg/mouse and was administered for 5 consecutivedays. These results suggest that a relatively high dose of SC-1225may be required to protect against in vivo infection, particularlywhen the MAb is usedalone.

We and other investigators reported that inflammatory cytokines, especially TNF- $alpha$ , IL-1 $beta$ , and IL-6, play important roles inthe pathological manifestations of septic shock (1, 27).These cytokines are also thought to be good markers of the severityof infection during bacterial infections (11, 24, 31). Therefore,we determined the levels of these cytokines in mice after gut-derivedsepsis, and the results demonstrated significant decreases inTNF- $alpha$ and IL-6 levels in antiflagellar MAb-treated mice in comparisonwith those in BSA-treated control mice. These results indicatethat antiflagellar MAb treatment ameliorates the P. aeruginosainfection and then influences cytokineproduction.

We have previously reported that blood culture-derived isolates are more virulent in the murine gut-derived sepsis model thanother clinical isolates of P. aeruginosa (16) and that the meanmotility of P. aeruginosa blood-derived isolates is significantlyhigher than that of sputum-derived isolates (19). Furthermore,infection with high-motility strains of P. aeruginosa resultsin significantly higher mortality rates than infection with low-motilitystrains in our murine gut-derived sepsis model (19). In thisreport we demonstrated the protective effect of antiflagellarhuman MAb SC-1225 against gut-derived sepsis caused by P. aeruginosa,and one of the protective mechanisms is suspected to be its opsonophagocyticactivity. We therefore conclude that the flagella of P. aeruginosaplay an important role in the gut-derived sepsis caused by thisorganism.

	ACKNOWLEDGMENTS

We are grateful to Shogo Kuwahara for useful advice and to Yasuko Kaneko for expert technicalassistance.

This work was supported by a research grant provided by The Japan Health Sciences Foundation, Tokyo,Japan.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Microbiology, Toho University School of Medicine, 5-21-16 Omori-Nishi,Ota-ku, Tokyo 143-8540, Japan. Phone: 81-3-3762-4151, ext. 2396.Fax: 81-3-5493-5415. E-mail: tetsu{at}med.toho-u.ac.jp.

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Abstract
Introduction
Materials and Methods
Results
Discussion
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28. Ochi, H., H. Ohtsuka, S. Yokota, I. Uezumi, M. Terashima, K. Irie, and H. Noguchi. 1991. Inhibitory activity on bacterial motility and in vivo protective activity of human monoclonal antibodies against flagella of Pseudomonas aeruginosa. Infect. Immun. 59:550-554[Abstract/Free Full Text].

29. Oishi, K., F. Sonoda, A. Iwagaki, P. Ponglertnapagorn, K. Watanabe, T. Nagatake, A. Siadak, M. Pollack, and K. Matsumoto. 1993. Therapeutic effects of a human antiflagella monoclonal antibody in a neutropenic murine model of Pseudomonas aeruginosa pneumonia. Antimicrob. Agents Chemother. 37:164-170[Abstract/Free Full Text].

30. Pennington, J. E., G. J. Small, M. E. Lostrom, and G. B. Pier. 1986. Polyclonal and monoclonal antibody therapy for experimental Pseudomonas aeruginosa pneumonia. Infect. Immun. 54:239-244[Abstract/Free Full Text].

31. Puren, A. J., C. Feldman, N. Savage, P. J. Becker, and C. Smith. 1995. Patterns of cytokine expression in community-acquired pneumonia. Chest 107:1342-1349[Abstract/Free Full Text].

32. Richardson, J. D., M. M. DeCamp, R. N. Garrison, and D. E. Fry. 1982. Pulmonary infection complicating intra-abdominal sepsis: clinical and experimental observations. Ann. Surg. 195:732-738[Medline].

33. Rosok, M. J., M. R. Stebbins, K. Connelly, M. E. Lostrom, and A. W. Siadak. 1990. Generation and characterization of murine antiflagellum monoclonal antibodies that are protective against lethal challenge with Pseudomonas aeruginosa. Infect. Immun. 58:3819-3828[Abstract/Free Full Text].

34. Sawada, S., T. Kawamura, and Y. Masuho. 1987. Immunoprotective human monoclonal antibodies against five major serotypes of Pseudomonas aeruginosa. J. Gen. Microbiol. 133:3581-3590[Medline].

35. Stoll, B. J., M. Pollack, L. S. Young, N. Koles, R. Gascon, and G. B. Pier. 1986. Functionally active monoclonal antibody that recognizes an epitope on the O side chain of Pseudomonas aeruginosa immunotype-1 lipopolysaccharide. Infect. Immun. 53:656-662[Abstract/Free Full Text].

36. Tamura, Y., S. Suzuki, and T. Sawada. 1992. Role of elastase as a virulence factor in experimental Pseudomonas aeruginosa infection in mice. Microb. Pathog. 12:237-244[Medline].

37. Tancrede, C. H., and A. O. Andremont. 1985. Bacterial translocation and gram-negative bacteremia in patients with hematological malignancies. J. Infect. Dis. 152:99-103[Medline].

38. Terashima, M., I. Uezumi, T. Tomio, M. Kato, K. Irie, T. Okuda, S. Yokota, and H. Noguchi. 1991. A protective human monoclonal antibody directed in the outer core region of Pseudomonas aeruginosa lipopolysaccharide. Infect. Immun. 59:1-6[Abstract/Free Full Text].

39. Uezumi, I., M. Terashima, T. Kohzuki, M. Kato, K. Irie, H. Ochi, and H. Noguchi. 1992. Effects of a human antiflagellar monoclonal antibody in combination with antibiotics on Pseudomonas aeruginosa infection. Antimicrob. Agents Chemother. 36:1290-1295[Abstract/Free Full Text].

40. Yokota, S., M. Terashima, J. Chiba, and H. Noguchi. 1992. Variable cross-reactivity of Pseudomonas aeruginosa lipopolysaccharide-code-specific monoclonal antibodies and its possible relationship with serotype. J. Gen. Microbiol. 138:289-296[Medline].

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Antimicrob. Agents Chemother.	Clin. Microbiol. Rev.	Infect. Immun.
J. Clin. Microbiol.	J. Virol.	ALL ASM JOURNALS

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28.	Ochi, H., H. Ohtsuka, S. Yokota, I. Uezumi, M. Terashima, K. Irie, and H. Noguchi. 1991. Inhibitory activity on bacterial motility and in vivo protective activity of human monoclonal antibodies against flagella of Pseudomonas aeruginosa. Infect. Immun. 59:550-554[Abstract/Free Full Text].
29.	Oishi, K., F. Sonoda, A. Iwagaki, P. Ponglertnapagorn, K. Watanabe, T. Nagatake, A. Siadak, M. Pollack, and K. Matsumoto. 1993. Therapeutic effects of a human antiflagella monoclonal antibody in a neutropenic murine model of Pseudomonas aeruginosa pneumonia. Antimicrob. Agents Chemother. 37:164-170[Abstract/Free Full Text].
30.	Pennington, J. E., G. J. Small, M. E. Lostrom, and G. B. Pier. 1986. Polyclonal and monoclonal antibody therapy for experimental Pseudomonas aeruginosa pneumonia. Infect. Immun. 54:239-244[Abstract/Free Full Text].
31.	Puren, A. J., C. Feldman, N. Savage, P. J. Becker, and C. Smith. 1995. Patterns of cytokine expression in community-acquired pneumonia. Chest 107:1342-1349[Abstract/Free Full Text].
32.	Richardson, J. D., M. M. DeCamp, R. N. Garrison, and D. E. Fry. 1982. Pulmonary infection complicating intra-abdominal sepsis: clinical and experimental observations. Ann. Surg. 195:732-738[Medline].
33.	Rosok, M. J., M. R. Stebbins, K. Connelly, M. E. Lostrom, and A. W. Siadak. 1990. Generation and characterization of murine antiflagellum monoclonal antibodies that are protective against lethal challenge with Pseudomonas aeruginosa. Infect. Immun. 58:3819-3828[Abstract/Free Full Text].
34.	Sawada, S., T. Kawamura, and Y. Masuho. 1987. Immunoprotective human monoclonal antibodies against five major serotypes of Pseudomonas aeruginosa. J. Gen. Microbiol. 133:3581-3590[Medline].
35.	Stoll, B. J., M. Pollack, L. S. Young, N. Koles, R. Gascon, and G. B. Pier. 1986. Functionally active monoclonal antibody that recognizes an epitope on the O side chain of Pseudomonas aeruginosa immunotype-1 lipopolysaccharide. Infect. Immun. 53:656-662[Abstract/Free Full Text].
36.	Tamura, Y., S. Suzuki, and T. Sawada. 1992. Role of elastase as a virulence factor in experimental Pseudomonas aeruginosa infection in mice. Microb. Pathog. 12:237-244[Medline].
37.	Tancrede, C. H., and A. O. Andremont. 1985. Bacterial translocation and gram-negative bacteremia in patients with hematological malignancies. J. Infect. Dis. 152:99-103[Medline].
38.	Terashima, M., I. Uezumi, T. Tomio, M. Kato, K. Irie, T. Okuda, S. Yokota, and H. Noguchi. 1991. A protective human monoclonal antibody directed in the outer core region of Pseudomonas aeruginosa lipopolysaccharide. Infect. Immun. 59:1-6[Abstract/Free Full Text].
39.	Uezumi, I., M. Terashima, T. Kohzuki, M. Kato, K. Irie, H. Ochi, and H. Noguchi. 1992. Effects of a human antiflagellar monoclonal antibody in combination with antibiotics on Pseudomonas aeruginosa infection. Antimicrob. Agents Chemother. 36:1290-1295[Abstract/Free Full Text].
40.	Yokota, S., M. Terashima, J. Chiba, and H. Noguchi. 1992. Variable cross-reactivity of Pseudomonas aeruginosa lipopolysaccharide-code-specific monoclonal antibodies and its possible relationship with serotype. J. Gen. Microbiol. 138:289-296[Medline].