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1	Utvärdering av fyra screeningmetoder för identifiering av kolistinresistens hos Escherichia coli och Klebsiella pneumoniae / Evaluation of four screening methods for the detection of colistin-resistant Escherichia coli and Klebsiella pneumoniae Axelsson, Emma January 2020 (has links) Multiresistens hos gramnegativa bakterier är ett stort problem i stora delar av världen. Avsaknaden av nya preparat har resulterat i återintroduktion av ett tidigare stoppat antibiotikum, kolistin, men dessvärre kantas resistensbestämningen av flertalet problem. Kolistin är en positivt laddad molekyl som binder till lipid A i yttermembranet, vilket destabiliseras och resulterar i celldöd. Flertalet resistensmekanismer mot kolistin finns beskrivna och majoriteten resulterar i förändrad lipid A-struktur, vilket leder till försämrad kolistininbindning. Syftet med examensarbetet var att utvärdera fyra potentiella screeningmetoder för att upptäcka kolistinresistens och jämföra resultaten mot buljongspädning som referensmetod. De fyra screeningmetoderna var buljongeluering och diskdiffusion samt de kommersiellt tillgängliga screeningtesterna Superpolymyxin och Rapid polymyxin NP. Totalt analyserades 57 helgenomsekvenserade Enterobacterales, varav 28 Escherichia coli och 29 Klebsiella pneumoniae, där aktuella resistensmekanismer var kända. Samtliga isolat analyserades en gång per metod och utöver detta analyserades även tre kontrollstammar. Vid buljongspädning erhölls värde för minsta inhiberande koncentration (MIC) kolistin, vilket användes för klassificering som känslig (MIC ≤ 2 mg/l) eller resistent (MIC > 2 mg/l). De fyra screeningtesterna var designade för att upptäcka resistenta isolat och innehöll 2–4 mg/l kolistin. Resultaten från screeningtesterna var kvalitativa och känslighetskategoriserade isolaten. Sensitivitet och specificitet beräknades för metoderna. Högst sensitivitet (100 %) noterades för Superpolymyxin och Rapid polymyxin NP, och lägst specificitet (76 %) för buljongeluering. Med hänsyn till resultat, prevalens, hållbarhets-, tids- och kostnadseffektivitet drogs slutsatsen att Rapid polymyxin NP är bästa alternativet som screeningmetod av utvärderade metoder. / Infections due to multidrug resistant Gram-negative bacteria are a major problem in large parts of the world. Due to lack of treatment options, a previously banned antibiotic, colistin, has been reintroduced. Unfortunately, susceptibility testing of colistin is problematic and currently the only recommended method is broth microdilution (BMD). Colistin is a positively charged molecule that binds to lipid A at the negatively charged outer cell membrane, which leads to cell disruption. Several mutations causing colistin resistance have been identified, most of them cause alterations of lipid A, resulting in impaired colistin outer cell membrane interaction. The aim of this study was to evaluate four potential screening methods for colistin resistance and compare the results with BMD (reference method). The four screening methods were broth disk elution, disk diffusion and the commercially available tests Superpolymyxin and Rapid polymyxin NP. A collection of 57 whole genome sequenced Enterobacterales consisting of 28 Escherichia coli and 29 Klebsiella pneumoniae were included in the study. Reference results were obtained by BMD, where the estimated minimum inhibitory concentration (MIC) values were used for classification of the isolates as sensitive (MIC ≤ 2 mg/l) or resistant (MIC > 2 mg/l). Sensitivity and specificity were calculated for the methods. The highest sensitivity (100 %) was noted for Superpolymyxin and Rapid polymyxin NP, and the lowest specificity (76 %) for broth disk elution. Considering the results, prevalence, durability, time and cost efficiency, it was concluded that Rapid polymyxin NP is the best alternative as a screening method of evaluated methods. Susceptibility testing broth microdilution colistin Antibiotikaresistensbestämning buljongspädning kolistin Microbiology Mikrobiologi
2	Histoplasma capsulatum: Drugs and Sugars Goughenour, Kristie 17 September 2020 (has links) No description available. Microbiology Histoplasma capsulatum Antifungals O-linked mannsylation susceptibility testing chitinases
3	Optimering av metod för upparbetning av Klebsiella pneumoniae från blododlingskultur inför flödescytometriassisterad resistensbestämning Hahlin, Emma January 2019 (has links) Under vissa omständigheter kan bakterier kan ta sig in i blodbanan där de kan orsaka allvarliga infektioner (bakteriemi). Metoden som används för identifiering och resistensbestämning av bakterier i blododlingar kräver minst 16 timmars inkubation. Fram tills en resistensbestämning utförts kan empirisk antibiotikabehandling användas, men med ökande resistensutbredning blir det alltmer osäkert om denna behandling är verksam. Nyligen har en lappdiffusionsmetod för resistensbestämning direkt från blododling validerats, som kan läsas av efter 4, 6 och/eller 8 timmars inkubation. Det finns även publicerade arbeten där flödescytometriassisterad resistensbestämning används, men då krävs att bakterierna finns i tillräckligt hög koncentration, befinner sig i tillväxtfas och finns som renkultur. Syftet med examensarbetet var att optimera hantering av blododlingsflaskor så att bakterier från blododlingsflaskorna kunde isoleras med tillräcklig kvalitet och koncentration för att kunna utföra resistensbestämning med flödescytometri. Upprening av bakterierna utfördes med olika tvättbuffertar och sedan utfördes resistensbestämning med flödescytometri och referensmetoden buljongspädning. Resultaten från uppreningen visade att sterilt vatten och Tween20 gynnade bakteriernas återhämtningsförmåga mest. Resistensbestämning utfördes med Klebsiella pneumoniae ATCC700603, K. pneumoniae CCUG56233 och K. pneumoniae ATCC13882, som tvättats med sterilt vatten och Tween20. För CCUG56233 skiljde 1 spädningssteg i koncentrationsskalan mellan metoderna. ATCC-isolaten erhöll likartade MIC-värden (minimum inhibitory concentration) vid alla analyser men där fanns en skillnad på 2 spädningssteg mellan buljongspädning och analys med flödescytometri. Detta kan förklaras av skillnaden i inkubationstid mellan metoderna. Slutsatsen som kan dras är därför att resultaten från de två metoderna vid resistensbestämning är likartade och att sterilt vatten är mest lämpligt att använda vid upprening av bakterier. Fler undersökningar bör dock utföras. Klebsiella pneumoniae flow cytometry antimicrobial susceptibility testing broth microdilution Klebsiella pneumoniae flödescytometri resistensbestämning buljongspädning Microbiology Mikrobiologi
4	CARBAPENEM-RESISTANT <em>ENTEROBACTERIACEAE</em>: EPIDEMIOLOGY, GENETICS, <em>IN VITRO</em> ACTIVITY, AND PHARMACODYNAMIC MODELING Kulengowski, Brandon 01 January 2019 (has links) Background: Infections caused by carbapenem-resistant Enterobacteriaceae (CRE) such as Escherichia coli and Klebsiella pneumoniae are among the most urgent threats of the infectious disease realm. The incidence of these infections has been increasing over the years and due to very limited treatment options, mortality is estimated at about 50%. By 2050, mortality from antimicrobial resistant infections is expected to surpass cancer at 10 million deaths annually. Methods: We evaluated 18 contemporary antimicrobials against 122 carbapenem-resistant Enterobacteriaceae using a variety of antimicrobial susceptibility testing methods according to Clinical Laboratory Standards Institute guidelines. Time-kill studies were performed on clinical isolates with variable resistance to meropenem, amikacin, and polymyxin B. Phenotypic expression assays were performed on all isolates and whole genome sequencing was performed on 8 isolates to characterize molecular resistance mechanisms. Pharmacodynamic modeling of meropenem and polymyxin B was also conducted. Results: CRE were primarily K. pneumoniae, and Enterobacter spp. 60% expressed Klebsiella pneumoniae carbapenemase (KPC) only, 16% expressed Verona Integron-encoded Metallo-beta-lactamase (VIM) only, 5% expressed KPC and VIM, and 20% expressed other mechanisms of resistance. Antimicrobial susceptibility testing indicated the most active antimicrobials against CRE were ceftazidime/avibactam, imipenem/relebactam, amikacin, tigecycline, and the polymyxins. Etest® strips did not reliably measure polymyxin B resistance. The automated testing system, BD Phoenix™, consistently reported lower MICs than the gold standard broth microdilution. Time-kill studies showed regrowth at clinically achievable concentrations of meropenem alone (4, 16, and 64 mg/L), polymyxin B alone (0.25 and 1 mg/L), or amikacin alone (8 and 16 mg/L), but combinations of meropenem with either polymyxin B or amikacin were bactericidal and synergistic. Meropenem administered simultaneously or prior to polymyxin B exhibited superior activity to polymyxin B administered first. Conclusions: Novel carbapenemase-inhibitor combinations (ceftazidime/avibactam and imipenem/relebactam) exhibit the best activity against KPC-producing CRE. The polymyxins, amikacin, and tigecycline exhibit the best activity against VIM-producing CRE. Meropenem in combination with polymyxin B is bactericidal and synergistic when the meropenem MIC is ≤32 mg/L, and meropenem should never be administered after polymyxin B. Meropenem and amikacin is bactericidal and synergistic when the amikacin MIC is ≤16 mg/L. Etest® strips should not be used for characterizing polymyxin B or colistin activity. Clinicians should be aware that automated testing systems may produce biased susceptibility results relative to the gold standard method, broth microdilution, which may influence interpretation of in vitro results. Carbapenem-resistant Enterobacteriaceae antimicrobial susceptibility testing time-kill whole-genome sequencing pharmacodynamic modeling Pharmacy and Pharmaceutical Sciences
5	Instantaneous Antimicrobial Susceptibility Testing Using Piezoelectric Sensors Aline M Elquist (7026050) 16 October 2019 (has links) Rapid determination of drugs effective against bacterial strains is critically important to stopping further spread of an infection and reducing antibiotic resistance. Antimicrobial susceptibility testing (AST) is done to determine what type of antibiotic and what concentration will be effective in treating an infection. Current, growth-dependent, AST methods are reliant on the growth rate of the bacteria and can take several days to several weeks to get results. A piezoelectric plate sensor can be used to measure an instant change in the minute physiological stresses of the bacteria cells when they are exposed to an effective concentration of antibiotic. This work aims to investigate the feasibility of piezoelectric plate sensors used for instantaneous AST (iAST) results and develop a technological framework for scaling this technology to a clinical lab setting. Four Clinical and Laboratory Standards Institute (CLSI) quality control strains of bacteria were tested with a wide range of antibiotics from various drug classes using the piezoelectric sensor. Results were obtained within 30 minutes and compared to standard of care AST methods used in clinical labs, and CLSI prescribed ranges for each strain of bacteria. This thesis will also discuss a framework for developing more scalable sensors, and challenges associated with the different sensor designs. Medical Devices piezoelectric antimicrobial susceptibility testing lead zirconate titanate Sensing Technology
6	A Hybrid Electrokinetic Bioprocessor For Single-Cell Antimicrobial Susceptibility Testing Lu, Yi January 2015 (has links) Infectious diseases resulting from bacterial pathogens are the most common causes of patient morbidity and mortality worldwide. The rapid identification of the pathogens and their antibiotic resistances is crucial for proper clinical management. However, the standard culture-based diagnostic approach requires a minimum of two days from the initial specimen collection to result reporting. As a consequence, broad-spectrum antibiotics are often prescribed under the worst-case assumption without knowledge of the pathogens or their resistances. The current clinical practice results in improper treatment of the patient and causes the rapid emergence of multi-drug resistant pathogens. A rapid diagnostics system has therefore been developed which performs hybrid electrokinetic sample preparation and volume reduction, for single-cell antimicrobial susceptibility testing (AST). The system combines multiple electrokinetic forces for sample preparation, which reduces the sample volume for over 3 orders of magnitude and minimizes the matrix effects of physiological samples for enhanced sensitivity. The device is integrated with a single-cell AST system with microfluidic confinement and electrokinetic loading to phenotypically determine the bacterial antibiotic resistance at the single-cell level. The applicability of the system has been demonstrated for performing direct AST with urine and blood samples within one hour, enabling rapid infectious disease diagnostics in non-traditional healthcare settings. antibiotic resistance antimicrobial susceptibility testing Electrokinetics microchannel single cell Mechanical Engineering AC electrothermal flow
7	Re-Evaluierung, methodische Optimierung und weitergehende Charakterisierung der Empfindlichkeitstestung von Mycobacterium tuberculosis mit dem BacT/Alert 3D (bioMérieux) Knigge, Anna Sophie 07 April 2014 (has links) (PDF) Es erfolgte die Re-Evaluierung der Empfindlichkeitstestung von Tuberkuloseerregern mit dem BacT/Alert-3D-System (bioMérieux) unter besonderer Berücksichtigung des Materialwechsels der Kulturflasche von Glas auf Plastik. Dazu wurden insgesamt 61 vergleichende MHK-Bestimmungen mit diesen beiden Flaschentypen durchgeführt, wobei sechs Antituberkulotika (INH, RMP, EMB, SM, PTH und MOX) sowie zwölf Mykobakterienstämme (davon neun Mtb.) untersucht wurden. Dabei findet sich kein Unterschied in den MHK-Werten zwischen Glas- und Plastikflaschen. Die Plastikflaschen sind folglich ebenso wie die Glasflaschen zur Empfindlichkeitstestung von Tuberkuloseerregern mit dem BacT/Alert-3D-System geeignet. Bei der bisherigen Methode wurde bei der PZA-Testung auf die Verwendung der Kontrollflasche zur Festlegung der Untersuchungszeit verzichtet, weil der erniedrigte pH-Wert ein unverhältnismäßig langsames oder gar fehlendes Wachstum in dieser Flasche bewirkt. Durch Optimierung von pH-Wert (pH 5,9) und PZA-Testkonzentration (200 mg/l) wurde erreicht, dass die PZA-Testung nach der gleichen Methode wie auch bei den anderen Antituberkulotika praktiziert, durchgeführt werden kann. Im weiteren wurde untersucht, wie hoch der Anteil resistenter Mutanten in Mischkulturen sein muss, um erkannt zu werden. Dazu wurden dem sensiblen Stamm H37Rv jeweils isogene Mutanten mit Monoresistenzen gegen INH, RMP oder SM bzw. EMB- und PZA-resistente Stämme in verschiedenen Anteilen zugesetzt. Es zeigte sich, dass ein Anteil von 1% resistenter Stämme noch nicht sicher detektiert wird. / The purpose of this paper is to optimize and reevaluate the methods of susceptibility testing of M.tuberculosis with the BacT/Alert 3D System (bioMérieux). The key aspect was the comparison between culture bottles from glass between those made out of plastic material. Therefore 61 comparative MIC-tests were carried out, with six antituberculous drugs (INH, RMP; EMB, SM, PTH and MOX) and twelve mycobacterial strains (nine Mtb.) in order to compare the MIC in the two different bottle types. The MIC of 40 comparative tests between plastic culture bottles were identical to those in glass material. Only 18 test results deviated between the two bottle types. In each of those tests the discrepancy was only one degree of dilution, which is considered as not relevant. Resistant strains were found in three tests, with no difference between glass and plastic bottles. The deviant twelve results of Mtb. strains show a six times higher MIC-value in plastic bottles and a six times lower MIC in plastic bottles. In the case of the substance INH all four discrepant results had a higher MIC in the plastic bottle. Since these results were known by the Institut für Medizinische Mikrobiologie und Infektionsepidemiologie of the University Leipzig, it was consequently used with good results in the laboratory routine, as well as in external quality control (INSTAND-Ringversuche 2009 to 2011). The second topic of this study was to optimize the current method of susceptibility testing of Mtb. concerning pyrazinamide (PZA). In the current method the low pH of the dilution (5.5) with the resulting weak growth of the strains forced the laboratory assistant to abandon the 1% control bottle as endpoint of measurement. The new and optimized pH of 5.9 and a concentration of PZA of 200 mg/l allows the susceptibility testing of PZA with the same method as practiced for the other antituberculous drugs. Yet another focus of this study was the sensitivity of the BacT/Alert 3D System to detect heteroresistant clones in the mycobacterial broth. Resistant clones and fully susceptible Mtb. strain (H37Rv) were mixed in different percentages and susceptibility testing was performed. It could be shown, that a secure detection of resistant clones is not possible at a percentage 1% of resistant clones in the culture. ddc:610
8	Avaliação da resistencia dos microrganismos colhidos no ambiente de clinica odontologica a diferentes antibioticos Pacheco, Aline de Barros Nobrega Dias 25 February 2000 (has links) Orientador: Thales Rocha de Mattos Filho / Dissertação (mestrado) - Universidade Estadual de Campinas, Faculdade de Odontologia de Piracicaba / Made available in DSpace on 2018-07-26T02:18:54Z (GMT). No. of bitstreams: 1 Pacheco_AlinedeBarrosNobregaDias_M.pdf: 5192338 bytes, checksum: 27b1c8a32fe10fca65e1b9c5c96f03b7 (MD5) Previous issue date: 2000 / Resumo: Deter a contaminação nos consultórios dentários tem sido uma tarefa muito difícil. Na maioria das vezes os microrganismos tem vencido as medidas de segurança adotadas, expondo profissionais e pacientes à situações de risco. Em escolas de Odontologia, esse risco é ainda maior, pois há dificuldades na implementação de procedimentos de controle de infecção. Para identificar os microrganismos do ambiente clínico de uma Faculdade de Odontologia e avaliar a resistência antimicrobiana desses, foi desenvolvida esta pesquisa. Para isso utilizou se 60 placas de petri (15 cm de diâmetro), contendo ágar-soja-triptecaseína, dispostas em diversos locais da clínica (box, corredor, sala de esterilização e plantão de urgência) e em três situações: antes, durante e após a atividade. As placas foram abertas (120 segundos) e então fechadas e levadas à estufa (pressão de CO2 a 10% à 37ºC), durante 48 horas, e então transferidas para uma estufa em aerobiose (37ºC), por mais 24 horas. As unidades formadoras de colônias que cresceram foram contadas e fotografadas, e para a identificação utilizou-se a técnica de coloração de Gram. A resistência foi avaliada em placas de petri contendo ágar Muller Hinton, acrescido de 1,5°/0 de sangue de carneiro estéril previamente inoculadas com 100 µL dos microrganismos, onde foram inseridos discos de papel de 6,35mm contendo antibióticos, e os halos de inibição, que se desenvolveram após incubação, foram medidos. A análise estatística (KrusKall Wallis, 5%) mostrou diferença significante durante as diversas situações clínicas. Observou-se ainda que, de todos os microrganismos, 26% foram resistentes à penicilina G 10UI, 18% à ampicilina 10g, 19% à amoxicilina 10µg, 6% à amoxicilina 10µg + ácido clavulânico 20µg, 7% ao cefadroxil 30µg, 27% à eritromicina 15µg, 25% à daritromicina 15µg, 27% à azitromicina 15µg, 14% à clindamicina 2µg e 3% ao cloranfenicol 30µg. Condui-se que: 1) Durante atividade clínica há um maior crescimento de microrganismos, prevalecendo cocos, bacilos e fungos respectivamente; 2) A resistência encontrada foi maior para os antibióticos do 9rupo dos macrolídeos (26,4%), seguida pelo grupo das penicilinas (21,1%), sendo que a amoxicilina associada ao ácido clavulânico e o doranfenicol apresentaram as menores resistências, 6,47% e 2,8%, respectivamente / Abstract: It has been a very hard task to stop contamination in dental clínies. Most of the times, microorganisms have beaten the preventive measures used exposing health practitioners and patients to risk situations. ln Dental Schools this risk becomes even higher, for three are difficulties implementing procedures of infection control. This research was carried out in order to identify the microorganisms in the dental clínica I environment of a Faculty of Dentistry, and also to evaluate their resistance. For this purpose, 60 petri dishes (15 cm of diameter) with tripticasein soy agar were placed on different places in the clinic environment (between the dental clínies, on the corridors, sterilization room and emergency room) in three different situations: before, during and after the clinical work. The dishes were opened during 120 seconds, and then closed and incubated (at 10% CO2 pression) at 37°C, during 48 hours, and after moved to a stove at 37°C for 24 hours. The colony formation units (du) that grew on the dishes were counted and photographed. The Gram coloring technique for identification was applied. The resistance was evaluated on petri dishes with Muller Hinton agar plus 1.5% sheep blood sterile, previously inoculated with 100µg of microorganisms, there paper disks of 6.35 mm with antibiotics were placed. After incubation, the halos, which developed, were measured. The statistical analysis (KrusKaIl-Wallis 5%) showed significant difference during the various clinical situations. It was observed that 26% of the microorganisms were resistant to penicillin G [10Ul], 18% to ampicillin [10µg], 6% to amoxycillin [10µg] associated with clavulanic acid [20µg], 7% to cefadroxil [30µg], 27% to erythromycin [15µg], 27% to azithromycin [15µg], 250% to clarithromycin [15µg], 14% to clyndamicin [2µg] and 3% to cloranphenicol [30µg]. Therefore, it was concluded that: a) During clinical work there is a higher growth of microorganisms, being the most predominant cocci, bacillus and fungus, respectively; b) The higher resistance found was to the antibiotics from the macrolides group (26%), followed by the penicillin group (21%), having amoxycillin associated with clavulanic acid and doranphenicol, showed the lowest resistance / Mestrado / Mestre em Odontologia Contaminação Testes microbiológicos Testes de sensibilidade bacteriana Infection control Environmental contamination Bacterial resistance Microbial susceptibility testing
9	Automatisation de la lecture et de l'interprétation des antibiogrammes / Automation of the reading and the interpretation of antibiotic susceptibility testing Le Page, Stéphanie 06 July 2017 (has links) Au cours des dernières années, l’automatisation en bactériologie clinique est devenue très importante du fait de l’augmentation constante du nombre d’échantillons mais nécessite tout de même des améliorations. Une revue a été rédigée pour présenter les nouveaux challenges et opportunités dans la surveillance et la détection des bactéries multi-résistantes. Premièrement nous avons testé de nouveaux outils technologiques innovants permettant la lecture plus précoce des antibiogrammes grâce à des scanners de haute résolution d’images: scanner Advencis Bio-System Incubator et le Scan® 1200 et de réaliser l’ensemencement des antibiogrammes en automatique sur un automate déjà existant le PREVI® Isola (bioMérieux, Marcy l’Etoile, France). Dans un second temps, une analyse rétrospective de la résistance aux antibiotiques observés sur l’hôpital la Timone à Marseille a été réalisé entre 2014 et 2016. Nous avons développer un logiciel d’interprétation automatique des phénotypes basé sur la reconnaissance d’images pour lequel un brevet a été rédigé : le logiciel « ANTI-LOGIC ». Le but de notre troisième travail a été de participer au développement d’une PCR en temps réel permettant de détecter le gène mcr-1. Puis, nous avons travaillé sur des souches multi-résistantes afin de tester un panel constitué de 29 à 32 antibiotiques. Pour la détection des souches résistantes à la colistine, un milieu de culture sélectif a été mis au point et nous avons essayé de trouver une alternative thérapeutique par l’étude de combinaisons d’anciens antibiotiques (colistine-sulfadiazine) pour le traitement et la décolonisation avant greffe fécale de patients infectés ou colonisés par des BMR. / In the last few years, automation in clinical microbiology has become very important due to the constant increase of samples but they need to be improved. A review of the literature was performed to expose the new challenges and the new opportunities in the surveillance and the detection of multi-drug resistance bacteria.For that purpose, we conduct a thorough search to test new innovative technological tools for reading earlier AST with high-resolution image scanner: Advencis Bio-System Incubator and the Scan® 1200 and to carry out the automatic seeding of AST with the PREVI® Isola system (bioMérieux, Marcy l’Etoile, France). In a second step, the retrospective analysis of antibiotic resistance and phenotypes observed at La Timone hospital in Marseille was carried out between 2014 and 2016. We have developped a new software for the automatic interpretation of phenotypes based on image recognition protected by a patent: the "ANTI-LOGIC" software. The aim of our third work was to participate on the development of a real-time PCR to detect the mcr-1 gene. We then worked on multi-resistant strains with Gram-negative bacteria, we have tested a large panel of 29-32 antibiotics to see if we are in a therapeutic stalemate. For the detection of colistin resistant strains, a selective culture medium has been developed. In order to finish this part, with the appearance of colistin-resistant strains, we tried to find a therapeutic alternative by studying combinations of old antibiotics (colistin-sulfadiazine) for the treatment and decolonization before faecal transplantation of patients infected or colonized by multi-resistant bacteria Automatisation Antibiogrammes Technologies innovantes Lecture plus précoce Automation Antibiotic susceptibility testing Innovatives technologies Earlier reading
10	Live single cell fluorescence microscopy; from antibiotic resistance detection to mitochondrial dysfunction Ray, Lucille Alexandria 26 August 2020 (has links) No description available. Biochemistry Chemistry Microbiology microscopy single-cell antibiotic resistance fluorescence mitochondria cuprizone antibacterial susceptibility testing antimicrobial polymer

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