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Quality Assurance of Antimicrobial Susceptibility Testing

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Dept of Clinical microbiology, V xj , Sweden ... Epidemic in the Lagan area. Quality Assurance. Standardisation/Calibration of method ... – PowerPoint PPT presentation

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Title: Quality Assurance of Antimicrobial Susceptibility Testing


1
Quality Assurance of Antimicrobial Susceptibility
Testing
  • Gunnar Kahlmeter
  • Dept of Clinical microbiology, Växjö, Sweden
  • The National Institute for Infectious Disease
    Control
  • SRGA SRGA-M, BSAC and EUCAST

2
Antimicrobial susceptibility testing is about
short-term and long-term credibility!Surprising
findings or trends will be questioned!
3
Standardisation/Calibration of method
Routine quality control
Quality Assurance
Education
Expert rules
Internal Quality Assessment (specimen
reprocessing)
External Quality Assessment
Adapted from Derek Brown
4
Standardisation and calibrationof method
  • Standardised methodology (BSAC, CA-SFM, DIN,
    NCCLS, SRGA)
  • QC-strains with target values
  • Reference MIC-distributions of wild type bacteria
    (on www.eucast.org)
  • Reference zone diameter distributions of wild
    type bacteria (on SRGA website and within the
    BSAC system)

5
E.coli ATCC 25922
Uppdaterad 2000-04-18
6
Reference MIC-distributions onwww.eucast.org
7
Reference MIC-distributions onwww.eucast.org
8
Reference zone diameter distributions
throughSRGA and BSAC
Data by Trevor Winstanley
9
Reference zone diameter distributions through
SRGA and BSAC
10
E.coli vs. gentamicin 30 µgn2478 from 17
countries
S/R 21/17
11
  • Discrepancies discovered in the validation
    procedure - analysis and suggested measures
  • - one or more of the distributions deviate from
    what is expected (the median is off, the
    distribution is wider than expected, the part of
    the distribution that ought to be unimodal is
    bimodal, etc) the pattern of the deviation can be
    used to diagnose the problem
  • are all basic parameters alike for the two
    histograms (disk strengths, additives,
    atmosphere, calibration of the CO2-incubator,
    temperature etc).
  • are species-identification procedures
    equivalent?
  • do the aberrations occur with media containing
    supplements? or with media or disks sensitive to
    storage? or with antibiotics sensitive to changes
    in pH (aminoglycoside, erythromycin)? or with
    antibiotics sensitive to the autoclaving of the
    medium (nitrofurantoin).

12
Zone diameter distributions from 4 Swedish
laboratories illustrating different
methodological outputs.
Reference SRGA distribution
Median
13
  • Discrepancies discovered in the validation
    procedure - analysis and suggested measures
  • If the majority of the distributions deviate from
    the expected there should be a pattern
  • inhibition zones smaller than the reference
    histograms inoculum too dense or incorrect agar
    volume in the plates (depth gt4 mm).
  • inhibition zones larger than the reference
    histograms incorrect agar volume in the plates
    (depth lt4 mm).

14
Standardisation/Calibration of method
Routine quality control
Quality Assurance
Education
Expert rules
Internal Quality Assessment (specimen
reprocessing)
External Quality Assessment
Adapted from Derek Brown
15
Routine quality control
  • QC-strains with target values (target values,
    permitted range, trend analysis in Shewart
    diagrams)- general overall proficiency check-
    specific rare organisms N.gonorrhoeae,
    H.pylorii, fungi etc
  • Serial analysis of zone diameter distributions
    (or MIC-distributions)

16
E.coli ATCC 25922
Uppdaterad 2000-04-18
17
Period of calibration
18
Variation attributable to the lab.technician (the
inoculum)
One of my oldest friends but her inocula were
always a bit too dense!
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21
Discrepancies in results with quality control
strains - analysis and remedies Random errors
cannot be avoided but shall be controlled.
Reference strains have been assigned target
values and acceptable intervals for random
variation. Occasional deviation can be accepted
but trends and recurring patterns should be
investigated, explained and corrected.
22
Discrepancies in results with quality control
strains - analysis and remedies Systematic errors
(systematic high or low values, or a trend)
should be investigated and corrected. - wrong
strain- disc content- volume of medium- pH of
medium - atmosphere and incubation
temperature)- aging of plates If this does not
explain and solve the problem the most probable
cause is the density of the inoculum.
23
A change in the ion-content of ISA (Oxoid)
24
Routine quality control
  • QC-strains with target values (target values,
    permitted range, trend analysis in Shewart
    diagrams)- general overall proficiency check-
    specific rare organisms N.gonorrhoeae,
    H.pylorii, fungi etc
  • Serial analysis of zone diameter distributions
    (or MIC-distributions)

25
Internal QA Serial analysis of zone diameter
distributions
The regular analysis of zone diameter
distributions of consecutive clinical
isolates provide good internal quality
asessment median (accuracy) width
(reproducibility) shape (tells you all sorts of
things about the drug, species, lab)
26
A high degree of reproducibility! A high degree
of credibility!
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28
Epidemic in the Lagan area
29
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30
Standardisation/Calibration of method
Routine quality control
Quality Assurance
Education
Expert rules
Internal Quality Assessment (specimen
reprocessing)
External Quality Assessment
Adapted from Derek Brown
31
Expert rules are an important part of
QA Penicillin resistance does not exist in
S.pyogenes- faulty disk Ampicillin resistance
in E.faecalis is very rare- erroneous species
identification Methicillinresistance in
Staphylococci should not permit an S for other
betalactam antibiotics- dont do them youll
get it wrong! Mistrust clarithromycin S if
erythromycin R- someone got the breakpoint
wrong
32
Standardisation/Calibration of method
Routine quality control
Quality Assurance
Education
Expert rules
Internal Quality Assessment (specimen
reprocessing)
External Quality Assessment
33
External Quality Assessment
  • The distribution of strains with known
    antimicrobial resistancies or MIC-values
  • - NEQAS, EQUALIS, RING, LABKA etc
  • - panel of experts to chose strains and to make
    the analysis of results and prepare comments
  • The analysis of yearly distributions of the
    quantitative results of consecutive clinical
    isolates combined EQA and resistance
    surveillance.

34
EQA in NEQAS and EARSS- please refer to NEQAS
and EARSS reports
35
Sweden
  • 100 consecutive patient isolates per bacterium
    and antibiotic and year and lab.
  • Each lab enter zone diameters over internet.
  • QA - the distributions are compared (median,
    width, scew) with reference.
  • Resistance surveillance - using SRGA breakpoints
    the resistance frequencies calculated and
    tabulated

36
S/R 18/17
  • Each laboratory is asked to test 100 consecutive
    patient strains of defined species (3 - 5)
    against defined antibiotics (4 - 6).
  • The zones are entered over the internet (see
    www.srga.org)
  • 30 labs x 100 strains 3000 strains per species
    antibiotic year with good geographical
    distribution.

37
ResNet
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