Activity of moxifloxacin against Bacteroides fragilis and Escherichia coli in an in vitro pharmacokinetic/pharmacodynamic model employing pure and mixed cultures

doi:10.1099/jmm.0.45994-0

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Activity of moxifloxacin against Bacteroides fragilis and Escherichia coli in an in vitro pharmacokinetic/pharmacodynamic model employing pure and mixed cultures

Reiner Schaumann¹, Ellie JC Goldstein², Jochen Forberg³ and Arne C Rodloff¹

¹Institute for Medical Microbiology and Epidemiology of Infectious Diseases, University of Leipzig, Leipzig, Germany ²R. M. Alden Research Laboratories, Santa Monica, CA 90404, USA ³Institute for Medical Informatics, Statistics and Epidemiology, University of Leipzig, Leipzig, Germany

Correspondence Reiner Schaumann schaur{at}medizin.uni-leipzig.de

Received December 22, 2004
Accepted May 23, 2005

The objective of this study was to determine the pharmacodynamic(PD) activity of moxifloxacin against four selected Bacteroidesfragilis strains (three strains with low MICs and one strainwith a high MIC) and two Escherichia coli strains (one strainwith a low MIC and one strain with a high MIC) in a pharmacokinetic(PK) in vitro model in pure cultures as well as in mixed cultures.PK/PD assays of moxifloxacin were carried out with an initialmaximum concentration of 4.0 mg l^–1 and a half-life of13 h. The E. coli strain with the low MIC was rapidly killedin both pure and mixed cultures in the in vitro PK/PD model,while the E. coli strain with the high MIC was not killed. Noneof the B. fragilis strains were rapidly killed in pure or mixedcultures. The bacterial numbers of the B. fragilis strains withlow MICs were reduced by about one to two logs after 12 h inpure cultures. The presence of an E. coli strain with a lowor a high MIC in the mixed culture reduced this effect evenfurther.

Abbreviations: PD, pharmacodynamic; PK, pharmacokinetic.

INTRODUCTION

TOP
INTRODUCTION
METHODS
RESULTS AND DISCUSSION
ACKNOWLEDGEMENTS
REFERENCES

Obligately anaerobic bacteria comprise the largest part of thephysiological flora on skin and mucous membranes of humans.Since they are opportunistic pathogens, they often participatein endogenous infections, causing mixed infections togetherwith aerobic bacteria. Such infections (i.e. intra-abdominal)are burdened with high morbidity and mortality, and requiretreatment with antimicrobial drugs showing activity againstboth aerobic and anaerobic bacteria (Gorbach, 1994; Nathens & Rotstein, 1996;Olsen et al., 1999).

Moxifloxacin is a quinolone that, like trovafloxacin and clinafloxacin,belongs to the fluoroquinolone group IV as defined by Naber & Adam (1998).It has an antimicrobial activity againstmany Gram-positive and Gram-negative aerobic and anaerobic bacteriaas well as atypical bacteria such as Chlamydia and Mycoplasma(Dalhoff et al., 1996; Bauernfeind, 1997; Goldstein et al., 1997;Edlund et al., 1998; Ackermann et al., 2000; Blondeau et al., 2000;Schaumann et al., 2000; Kleinkauf et al., 2001;Krasemann et al., 2001; Talan, 2001; Zhanel et al., 2002).

Several in vitro studies have indicated that moxifloxacin hasgood in vitro activity against important anaerobic bacteriaespecially Bacteroides species (Edlund et al., 1998; Ackermann et al., 2000).However, compared to the activities of garenoxacin,clinafloxacin, sitafloxacin and trovafloxacin, moxifloxacinmore recently was the least active agent against 589 Bacteroidesfragilis group isolates (Snydman et al., 2002). Furthermore,fluoroquinolone resistance among Bacteroides isolated in theUSA has apparently markedly increased since 1994 (Golan et al., 2003).Hedberg & Nord (2003) reported that antimicrobialresistance among B. fragilis group isolates in Europe is alsoincreasing. Conversely, cidal moxifloxacin activity was foundfor respiratory pathogens (aerobes and anaerobes) even whensera were obtained 24 h after dosing. The results suggest thatmoxifloxacin may have clinical utility in the treatment of mixedaerobic/anaerobic respiratory tract infections (Stein et al., 2003b).In a recently published paper investigating serum bactericidalactivity of moxifloxacin and gatifloxacin, Stein et al. (2003a)reported little or no serum bactericidal activity of eitherdrug if the MICs of gatifloxacin were $>=$ 2 mg l^–1. However,moxifloxacin was found to be effective in vivo even againsta B. fragilis strain with a high MIC level for moxifloxacinin an experimental animal model of severe mixed aerobic/anaerobicinfection (Schaumann et al., 2004).

The aim of the present study was to assess the killing activityof moxifloxacin in an in vitro pharmacokinetic/pharmacodynamic(PK/PD) model against four selected B. fragilis strains usedpreviously in the in vivo experimental model (Schaumann et al., 2004).Since anaerobes are often present in mixed infections,kill kinetics were also established for mixed inocula employingthe B. fragilis strains together with one of two different Escherichiacoli strains, one strain with a low MIC for moxifloxacin andone with a high MIC.

METHODS

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INTRODUCTION
METHODS
RESULTS AND DISCUSSION
ACKNOWLEDGEMENTS
REFERENCES

Bacterial strains.

E. coli ATCC 25922, E. coli VA 6886 and different strains ofB. fragilis (RMA 0309, RMA 5120, RMA 6791, WAL R 13267) wereused. E. coli VA 6886 was isolated from bile at the Instituteof Medical Microbiology of Leipzig, Germany. RMA 0309 and RMA5120 were intra-abdominal isolates, RMA 6791 was a blood cultureisolate and WAL R 13267 was a clinical isolate of unknown origin.

The B. fragilis strains and E. coli ATCC 25922 strain were characterizedas follows as described previously (Schaumann et al., 2004):B. fragilis RMA 0309, enterotoxin negative, MIC for moxifloxacin0.125 mg l^–1; B. fragilis RMA 5120, enterotoxin negative,MIC for moxifloxacin 0.125–0.38 mg l^–1; B. fragilisRMA 6791, enterotoxin positive, MIC for moxifloxacin 0.25–0.5mg l^–1; B. fragilis WAL R 13267, enterotoxin positive,MIC for moxifloxacin >32 mg l^–1; E. coli ATCC 25922,MIC value for moxifloxacin <0.03 mg l^–1.

The MIC for the E. coli strain VA 6886 was established by brothmicrodilution technique according to DIN 58940-8 (Deutsches Institut für Normung e.V., 2000).The result was confirmedby E-test (AB BIODISK) according to the manufacturer's instructions,resulting in a MIC value of >32 mg l^–1.

The E. coli strains were grown on Endo agar (bioMérieux)and the B. fragilis strains were grown on Columbia agar (Oxoid)supplemented with 5 % sheep blood (Oxoid), vitamin K1 (Sigma)and haemin (Serva Feinbiochemica). After incubation, B. fragilisstrains and E. coli strains were harvested from the plates andsuspended separately in Brucella broth (Becton Dickinson) supplementedwith vitamin K1 and haemin, and incubated overnight at 37 °Cunder anaerobic and aerobic conditions, respectively. Then thesuspensions were adjusted turbidimetrically to contain approximately1.2 x 10⁹ c.f.u. ml^–1 B. fragilis and approximately 1.5x 10⁸ c.f.u. ml^–1 E. coli. Cultures for the experimentalmodel were set up as described below and the numbers of bacteriawere confirmed by appropriate plating.

Antimicrobial agent.

Moxifloxacin powder of known activity was kindly provided byBayer Vital and suspended in distilled water.

Experimental model.

In order to determine the pharmacodynamic activity of moxifloxacinall six strains were investigated in pure cultures as well asin mixed cultures. Cultures were set up in a final volume of20 ml of appropriately supplemented Brucella broth with approximately2.4 x 10⁸ c.f.u. ml^–1 B. fragilis or approximately 3 x10⁷ c.f.u. ml^–1 E. coli or both, and an initial maximumconcentration (C_max) of 4.0 mg l^–1 moxifloxacin. The invitro pharmacokinetic assays for moxifloxacin were carried outover 12 h with t_1/2 of 13 h according to the equation C_t = C₀x e^{–kel x t} (C_t = concentration of moxifloxacin at a givenpoint in time (t); C₀ = initial concentration of moxifloxacin).The elimination rate constant (k_el) was calculated using theequation k_el = ln 2/t_1/2.

An observation time period of 12 h was chosen according to thehalf-life of moxifloxacin and the dosing interval suggestedfor intra-abdominal infections. We used a C_max concentrationfor moxifloxacin of 4 mg l^–1 equal to total concentrationsince protein binding of moxifloxacin probably occurs in culturemedia as well. High inocula of approximately 2.4 x 10⁸ c.f.u.ml^–1 B. fragilis and approximately 3 x 10⁷ c.f.u. ml^–1E. coli were used since abscesses contain a large number ofbacteria (Stearne et al., 2001 & 2002).

The PK/PD model was established by adding appropriate amountsof supplemented Brucella broth every 30 min (540–980 µl),resulting in a final volume of 36.25 ml and a final moxifloxacinconcentration of 2.11 mg l^–1 after 12 h. At 30 min intervalssamples (20 µl) were taken and diluted aliquots were platedon Endo agar as well as on supplemented Columbia agar. The experimentswere carried out in an anaerobic chamber (Heraeus) containing80 % N₂, 15 % CO₂ and 5 % H₂ at 37 °C. However, the Endoagar plates were incubated under aerobic conditions for 24 h.After incubation, bacterial colonies were counted and calculatedto colony forming units per ml. The detection limit was 1 x10² c.f.u. ml^–1. In mixed cultures it was macroscopicallypossible to distinguish the colonies of E. coli from the coloniesof B. fragilis strains growing on Columbia agar due to morphologicalcriteria.

Statistical analysis.

Mann trend test was used for testing for trends in a time-seriesof killing ratios (Hartung, 1999; Hollander & Wolfe, 1999).A P value of <0.05 was considered to be significant.

RESULTS AND DISCUSSION

TOP
INTRODUCTION
METHODS
RESULTS AND DISCUSSION
ACKNOWLEDGEMENTS
REFERENCES

For our PK/PD assay we employed a reasonably high initial concentrationof moxifloxacin (4 mg l^–1) that was reduced to approximately2.11 mg l^–1 after 12 h. In pure cultures the bacterialnumbers of B. fragilis strains with low MICs ( $<=$ 0.5 mg l^–1)were moderately but significantly reduced (by about one to twologs) by moxifloxacin within 12 h (killing rates: RMA 0309,99.3 %; RMA 5120, 99.2 %; RMA 6791, 99.2 %; P < 0.01). ForB. fragilis WAL R 13267 (MIC >32 mg l^–1) no reductionwas observed (P > 0.05). Thus, none of the B. fragilis strainswas effectively killed in pure culture (Fig. 1).

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Fig. 1. Activity of moxifloxacin against four different strains of B. fragilis tested in the in vitro PK/PD model in pure cultures with and without moxifloxacin. MXF+, with moxifloxacin; MXF–, control without moxifloxacin. Detection limit: 10² c.f.u. ml^–1.

The E. coli ATCC 25922 strain (MIC < 0.03 mg l^–1) wasrapidly killed by moxifloxacin both in pure (data not shown)and mixed cultures (Fig. 2a), confirming a bactericidal effectagainst this strain (P < 0.01; killing rate within the firsthour >99.9 %). As was to be expected, there was no bactericidaleffect of moxifloxacin against the E. coli strain VA 6886 (MICvalue: >32 mg l^–1) at the moxifloxacin concentrationsemployed here (Fig. 2b; P > 0.05; data of pure culture notshown).

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Fig. 2. Activity of moxifloxacin against four different strains of B. fragilis tested in the presence of (a) E. coli strain ATCC 25922 (low MIC for moxifloxacin) and (b) E. coli strain VA 6886 (high MIC for moxifloxacin) in the in vitro PK/PD model. MXF+, with moxifloxacin; MXF–, control without moxifloxacin; EC, E. coli ATCC 25922 in (a) or E. coli VA 6886 in (b). Detection limit: 10² c.f.u. ml^–1.

In mixed cultures employing E. coli strain ATCC 25922, withthe low moxifloxacin MIC, the bacterial numbers of B. fragilisstrains with low MICs were significantly reduced (killing rates:RMA 5120, 90.5 %; RMA 6791, 91.8 %; RMA 0309, 99.8 %; P <0.01; Fig. 2a) and the growth rate of the B. fragilis strainwith a high MIC (WAL R 13267) was significantly lower comparedto the control without moxifloxacin (P < 0.01). Nevertheless,in the presence of the E. coli strain ATCC 25922 the moderateactivity of moxifloxacin against the anaerobes (except strainRMA 0309) was significantly reduced as compared to single anaerobiccultures (P $<=$ 0.01). In mixed cultures containing the E. colistrain VA 6886 and the B. fragilis strains with low MICs, thebacterial numbers of these bacteria were again significantlyreduced compared to the control (killing rates: RMA 0309, 72.2%; RMA 5120, 82.7 %; RMA 6791, 88.2 %; P < 0.01; Fig. 2b)but significantly less reduced if compared to pure cultureswith moxifloxacin (P < 0.01). Comparing the effects of thetwo E. coli strains on the anaerobes a significant differencein killing was only found for B. fragilis RMA 0309 (P < 0.01).In addition, the growth of the B. fragilis WAL R 13267 strainwas significantly lower in the presence of the E. coli VA 6886strain when compared to pure culture or to the mixed culturewith E. coli ATCC 25922 (P < 0.01). However, the growth ofthe B. fragilis WAL R 13267 strain was not reduced by moxifloxacincompared to the initial inoculum.

In contrast to the moderate activity of moxifloxacin investigatedhere using the in vitro PK/PD model, moxifloxacin has been shownto be as efficacious as imipenem/cilastatin in the treatmentof severe systemic mixed aerobic/anaerobic infection in miceusing the same B. fragilis strains and E. coli strain ATCC 25922(Schaumann et al., 2004). Earlier observations of Onderdonk et al. (1976)suggested that E. coli is primarily responsiblefor the lethal effects in the animals. Therefore, the resultsof the PK/PD model support those previous observations sincein the in vitro PK/PD model, moxifloxacin was fully bactericidalagainst the E. coli strain ATCC 25922. The presence of the E.coli ATCC 25922 and VA 6886 strains reduced the killing activityof moxifloxacin against the B. fragilis strains investigatedin the in vitro PK/PD model. This observation is supported byearlier results obtain with trovafloxacin (Stearne et al., 2001).Furthermore, protection of B. fragilis against the activityof metronidazole by Enterococcus faecalis has also been observed(Nagy & Földes, 1991). Nagy & Földes (1991)reported that metronidazole was inactivated by a cell extractof E. faecalis. However, inactivation of trovafloxacin by Enterococcusfaecium was not described (Stearne et al., 2001).

The reason for the different killing rates of moxifloxacin againstthe B. fragilis strains with low MICs investigated in our PK/PDmodel in mixed cultures is not yet understood. Stearne et al. (2001)discussed whether the emergence and selection of trovafloxacin-resistantmutants, with possible transfer of this resistance to B. fragilisin mixed infections, could account for the protection againstthe activity of the antimicrobial agent. However, further investigationswould be required to confirm this hypothesis. Because of theresults reported here, the clinical study data obtained formoxifloxacin treatment of patients with intra-abdominal infectionsneed intensive scrutiny.

ACKNOWLEDGEMENTS

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INTRODUCTION
METHODS
RESULTS AND DISCUSSION
ACKNOWLEDGEMENTS
REFERENCES

This study was supported by a grant from Bayer Vital GmbH, Leverkusen,Germany. This work was presented in part at the 43rd InterscienceConference on Antimicrobial Agents and Chemotherapy, Chicago,IL, 14–17 September 2003.

REFERENCES

TOP
INTRODUCTION
METHODS
RESULTS AND DISCUSSION
ACKNOWLEDGEMENTS
REFERENCES

Ackermann, G., Schaumann, R., Pless, B., Claros, M. C., Goldstein, E. J. C. & Rodloff, A. C. (2000). Comparative activity of moxifloxacin in vitro against obligately anaerobic bacteria. Eur J Clin Microbiol Infect Dis 19, 228–232.[CrossRef][Medline]

Bauernfeind, A. (1997). Comparison of the antibacterial activities of the quinolones Bay 12-8039, gatifloxacin (AM 1155), trovafloxacin, clinafloxacin, levofloxacin and ciprofloxacin. J Antimicrob Chemother 40, 639–651.[Abstract/Free Full Text]

Blondeau, J. M., Laskowski, R., Bjarnason, J. & Stewart, C. (2000). Comparative in vitro activity of gatifloxacin, grepafloxacin, levofloxacin, moxifloxacin and trovafloxacin against 4151 Gram-negative and Gram-positive organisms. Int J Antimicrob Agents 14, 45–50.[CrossRef][Medline]

Dalhoff, A., Petersen, U. & Endermann, R. (1996). In vitro activity of BAY 12-8039, a new 8-methoxyquinolone. Chemotherapy 42, 410–425.[Medline]

Deutsches Institut für Normung e.V. (2000). Medizinische Mikrobiologie und Immunologie: Diagnostische Verfahren, 3rd edn. Berlin/Wien/Zürich: Beuth.

Edlund, C., Sabouri, S. & Nord, C. E. (1998). Comparative in vitro activity of BAY 12-8039 and five other antimicrobial agents against anaerobic bacteria. Eur J Clin Microbiol Infect Dis 17, 193–195.[Medline]

Golan, Y., McDermott, L. A., Jacobus, N. V. & 11 other authors (2003). Emergence of fluoroquinolone resistance among Bacteroides species. J Antimicrob Chemother 52, 208–213.[Abstract/Free Full Text]

Goldstein, E. J. C., Citron, D. M., Hudspeth, M., Hunt Gerardo, S. & Merriam, V. (1997). In vitro activity of Bay 12-8039, a new 8-methoxyquinolone, compared to the activities of 11 other oral antimicrobial agents against 390 aerobic and anaerobic bacteria isolated from human and animal bite wound skin and soft tissue infections in humans. Antimicrob Agents Chemother 41, 1552–1557.[Abstract]

Gorbach, S. L. (1994). Antibiotic treatment of anaerobic infections. Clin Infect Dis 18 Suppl. 4, S305–S310.

Hartung, J. (1999). Statistik: Lehr- und Handbuch der angewandten Statistik, 12th edn. München/Wien/Oldenbourg: R. Oldenbourg Verlag.

Hedberg, M. & Nord, C. E. on behalf of the ESCMID Study Group on Antimicrobial Resistance in Anaerobic Bacteria (2003). Antimicrobial susceptibility of Bacteroides fragilis group isolates in Europe. Clin Microbiol Infect 9, 475–488.[CrossRef][Medline]

Hollander, M. & Wolfe, D. A. (1999). Nonparametric Statistical Methods, 2nd edn. New York: Wiley.

Kleinkauf, N., Ackermann, G., Schaumann, R. & Rodloff, A. C. (2001). Comparative in vitro activities of gemifloxacin, other quinolones, and nonquinolone antimicrobials against obligately anaerobic bacteria. Antimicrob Agents Chemother 45, 1896–1899.[Abstract/Free Full Text]

Krasemann, C., Meyer, J. & Tillotson, G. (2001). Evaluation of the clinical microbiology profile of moxifloxacin. Clin Infect Dis 32 Suppl. 1, S51–S63.

Naber, K. G. & Adam, D. unter Mitwirkung einer Expertengruppe der Paul-Ehrlich-Gesellschaft für Chemotherapie e V. (1998). Einteilung der Fluorchinolone. Chemotherapie J 7, 66–68.

Nagy, E. & Földes, J. (1991). Inactivation of metronidazole by Enterococcus faecalis. J Antimicrob Chemother 27, 63–70.[Abstract/Free Full Text]

Nathens, A. B. & Rotstein, O. D. (1996). Antimicrobial therapy for intraabdominal infection. Am J Surg 172 Suppl. 6A, 1S–6S.[CrossRef]

Olsen, I., Solberg, C. O. & Finegold, S. M. (1999). A primer on anaerobic bacteria and anaerobic infections for the uninitiated. Infection 27, 159–165.[Medline]

Onderdonk, A. B., Bartlett, J. G., Louie, T., Sullivan-Seigler, N. & Gorbach, S. L. (1976). Microbial synergy in experimental intra- abdominal abscess. Infect Immun 13, 22–26.[Abstract/Free Full Text]

Schaumann, R., Ackermann, G., Pless, B., Claros, M. C., Goldstein, E. J. C. & Rodloff, A. C. (2000). In vitro activities of fourteen antimicrobial agents against obligately anaerobic bacteria. Int J Antimicrob Agents 16, 225–232.[CrossRef][Medline]

Schaumann, R., Blatz, R., Beer, J., Ackermann, G. & Rodloff, A. C. (2004). Effect of moxifloxacin versus imipenem/cilastatin treatment on the mortality of mice infected intravenously with different strains of Bacteroides fragilis and Escherichia coli. J Antimicrob Chemother 53, 318–324.[Abstract/Free Full Text]

Snydman, D. R., Jacobus, N. V., McDermott, L. A. & 10 other authors (2002). In vitro activities of newer quinolones against Bacteroides group organisms. Antimicrob Agents Chemother 46, 3276–3279.[Abstract/Free Full Text]

Stearne, L. E. T., Kooi, C., Goessens, W. H. F., Bakker-Woudenberg, I. A. J. M. & Gyssens, I. C. (2001). In vitro activity of trovafloxacin against Bacteroides fragilis in mixed culture with either Escherichia coli or a vancomycin-resistant strain of Enterococcus faecium determined by an anaerobic time-kill technique. Antimicrob Agents Chemother 45, 243–251.[Abstract/Free Full Text]

Stearne, L. E. T., Buijk, S. L., Mouton, J. W. & Gyssens, I. C. (2002). Effect of a single percutaneous abscess drainage puncture and imipenem therapy, alone or in combination, in treatment of mixed-infection abscesses in mice. Antimicrob Agents Chemother 46, 3712–3718.[Abstract/Free Full Text]

Stein, G. E., Schooley, S. & Kaatz, G. W. (2003a). Serum bactericidal activity of the methoxyfluoroquinolones gatifloxacin and moxifloxacin against clinical isolates of Staphylococcus species: are the susceptibility breakpoints too high? Clin Infect Dis 37, 1392–1395.[CrossRef][Medline]

Stein, G. E., Schooley, S., Tyrrell, K. L., Citron, D. M. & Goldstein, E. J. C. (2003b). Bactericidal activities of methoxyfluoroquinolones gatifloxacin and moxifloxacin against aerobic and anaerobic respiratory pathogens in serum. Antimicrob Agents Chemother 47, 1308–1312.[Abstract/Free Full Text]

Talan, D. A. (2001). Clinical perspectives on new antimicrobials: focus on fluoroquinolones. Clin Infect Dis 32 Suppl. 1, S64–S71.

Zhanel, G. G., Ennis, K., Vercaigne, L., Walkty, A., Gin, A. S., Embil, J., Smith, H. & Hoban, D. J. (2002). A critical review of the fluoroquinolones: focus on respiratory infections. Drugs 62, 13–59.[CrossRef][Medline]

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