All are true about ESBL except -

Classification is based on 3rd generation cephalosporin sensitivity

Cephalosporin sensitivity testing is required to confirm ESBL

Ambler classification is based on molecular structure

All of the following are true about methicillin resistance in MRSA, except:

Resistance is primarily mediated/transmitted by plasmids

Resistance is produced as a result of altered PBPs

Resistance may be missed at incubation temperature of 37°C during susceptibility testing

Resistance is associated with increased minimum inhibitory concentrations (MICs) for beta-lactam antibiotics

Which of the following is NOT a criterion for defining extensively drug-resistant tuberculosis (XDR-TB)?

Isoniazid + Rifampicin + Fluoroquinolone

Isoniazid + Rifampicin + Ethambutol + Fluoroquinolone

Isoniazid + Rifampicin + Kanamycin

Organism showing marked resistance to multidrug therapy -

Calymmatobacterium granulomatosis

Detection of Antimicrobial Resistance for FMGE: High-Yield Microbiology Lessons

Phenotypic Intro - Resistance Spotting 101

Phenotypic methods: Detect antimicrobial resistance (AMR) by observing bacterial growth response to antibiotics.
Core principle: "Sees" if bacteria can grow (resistant) or are inhibited/killed (susceptible) by a drug.
Directly measures the expressed resistance; what the drug actually encounters in the patient.
Often considered the reference standard for guiding clinical therapy.
Major categories:
- Disk Diffusion (e.g., Kirby-Bauer): Measures zone of inhibition size.
- Dilution (Broth/Agar): Determines Minimum Inhibitory Concentration (MIC).
- Automated Systems: Provide rapid, standardized results.
Pros: Clinically intuitive, generally cost-effective.
Cons: Slower (requires bacterial growth), some resistance mechanisms (e.g., inducible clindamycin resistance) may require specific tests.

⭐ The Minimum Inhibitory Concentration (MIC) is the lowest concentration of an antimicrobial that inhibits visible growth of a microorganism after overnight incubation; a cornerstone of susceptibility testing.

Diffusion/Dilution - Zone & MIC Workhorses

Phenotypic methods: Observe growth inhibition by antimicrobials.
Disk Diffusion (Kirby-Bauer)
- Principle: Antibiotic diffuses from disk into agar.
- Measures: Zone of Inhibition (ZOI) diameter (mm).
- Interpretation: ZOI correlates to S/I/R (CLSI/EUCAST).
- Qualitative/Semi-quantitative.
Dilution Methods (Broth/Agar)
- Principle: Organism vs. serial antibiotic dilutions.
- Determines: Minimum Inhibitory Concentration (MIC) - lowest concentration inhibiting visible growth.
- Quantitative.
- Broth microdilution: Common (96-well plates).
MIC: Crucial for therapy; guides dosage.

⭐ MIC is the lowest concentration of an antimicrobial that inhibits visible growth of a microorganism in vitro.
MBC (Minimum Bactericidal Concentration): Lowest concentration killing ≥99.9% of initial inoculum.

Targeted Phenotypic Tests - Superbug Unmasking

MRSA (Methicillin-Resistant S. aureus)
- Cefoxitin disc (30µg): Zone ≤ 21mm for S. aureus.
- PBP2a detection (e.g., latex agglutination, chromogenic agar).
VRE (Vancomycin-Resistant Enterococci)
- Vancomycin screen agar (6 µg/ml vancomycin).
ESBL (Extended-Spectrum β-Lactamase) Producers
- Screen: Resistance to 3rd gen cephalosporins (e.g., Cefotaxime, Ceftazidime).
- Confirm: Combination Disc Test (CDT) - Ceftazidime/Cefotaxime ± Clavulanate (zone difference ≥ 5mm).
AmpC β-Lactamase
- Cefoxitin resistance.
- AmpC disc test / Cloxacillin synergy test.
Carbapenemase Producers (CPE)
- Screen: Carbapenem resistance (Ertapenem most sensitive indicator).
- Confirm: mCIM (zone 6-15mm or pinpoint colonies); eCIM for MBLs (zone difference ≥ 5mm with EDTA).

Flowchart diagram

Workflow for rapid antimicrobial resistance detection

⭐ The mCIM test is crucial for detecting carbapenemase activity, and eCIM helps differentiate Metallo-β-Lactamases (MBLs) using EDTA. This has largely replaced the less specific Modified Hodge Test (MHT).

Genotypic & Novel Methods - Gene Code Crackers

Genotypic Methods: Directly detect resistance genes or mutations.
- PCR & Real-time PCR: Rapid; targets specific genes (e.g., mecA, vanA, blaKPC, mcr-1).
- DNA Microarrays/Multiplex Panels: Simultaneous detection of multiple resistance genes.
- Whole Genome Sequencing (WGS): Comprehensive; identifies known/novel mechanisms, crucial for outbreak epidemiology.
- Advantages: Fast (hours), culture-independent, not affected by prior antibiotic use.
- Limitation: Gene presence ≠ expression of resistance.
Novel & Rapid Phenotypic Methods:
- MALDI-TOF MS: Detects antibiotic degradation (e.g., β-lactamase activity by identifying hydrolyzed antibiotic peaks).
- Bacteriophage-based assays: Use phage lysis or reporter systems for rapid susceptibility.

⭐ Detection of the mecA gene by PCR is a cornerstone for identifying Methicillin-Resistant Staphylococcus aureus (MRSA).

High‑Yield Points - ⚡ Biggest Takeaways

Phenotypic methods: Kirby-Bauer (disk diffusion) and MIC determination (E-test, dilution) are key.

Genotypic methods (PCR) detect resistance genes like mecA (MRSA) and vanA (VRE).

ESBLs detected by double-disk synergy (DDST) or combination disk tests (ceftazidime + clavulanate).

Carbapenemase detection: Carba NP test (preferred) or Modified Hodge Test (MHT).

Cefoxitin disk diffusion is the recommended screening for MRSA.

D-test detects inducible clindamycin resistance in staphylococci (iMLS_B).

Automated systems (VITEK) provide rapid MICs and resistance profiles.

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