4. Diagnostic Techniques Flashcards

1
Q

Size of VIRUS + what microscope used?

A

Virus: 0.03-0.3 microns, use electron & light microscope

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2
Q

Size of BACTERIA + what microscope used?

A

Bacteria: 0.1-10 microns, light microscope

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3
Q

Size of MICROSCOPIC PROTOZOA & FUNGI + what microscope used?

A

Microscopic protozoa & fungi: 4-40 microns, light microscope

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4
Q

Membrane pore size that filters out bacteria:

A

0.4 microns (μm)

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5
Q

Resolution of microscopes of 1. Electron 2. Light 3. Human eye

A

Electron: 0.003 microns
Light: 0.2 microns
Human eye: 40 microns

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6
Q

Why do we use microscopy?

A
  1. Microscopy (of original sample) is faster than culturing the bacteria (culturing takes time)
  2. Some microbes cannot be cultured
  3. Make ‘best guess’ to guide therapy
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7
Q

Stains used in microscopy:

A
  1. Gram stain (for most bacteria)
  2. Ziehl Neelsen (usually to detect mycobacteria, stained reddish)
  3. Immunoflorescence
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8
Q

What are the 5 bacteriological investigations commonly used?

A
  1. Microscopy
  2. Culture
  3. Serology (antibody)
  4. Antigen detection
  5. PCR: polymerase chain reaction
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9
Q

Culture gives more information than microscopy:

A
  1. Definitive identification
  2. Antibiotic sensitivity testing
  3. Typing
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10
Q

What is MALDI-TOF

A

MALDI-TOF is a mass spectrometry method used to identify most bacteria in the clinical laboratory (via peptides/proteins)

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11
Q

What is Ziehl Neelson Stain usually used for?

A
  • used to detect Mycobacterium species (aka acid fast bacilli) => it causes TB
  • Mycolic acid in its cell wall => acid-fastness (resistance to decolourisation by acids => retains stain)
  • doesn’t let any gram stain in
  • reddish on histo slide
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12
Q

Steps to using Ziehl Neelson Stain:

A
  1. Bacteria stained w hot carbol fuchsin
  2. Decolourisation using acid-alcohol + wash
    - most bacteria lose stain BUT cell walls of Mycobacteria retain stain (APPEARS PINKISH/REDDISH)
  3. Counterstain (to see other bacteria)

ZN stain used to identify acid-fast bacilli (AFB)

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13
Q

IgG and IgM in primary and secondary infection.

A

IgM: prominent in primary infection, less common in secondary infection

IgG: takes times to appear in primary infection, much more prominent in secondary infection

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14
Q

Serodiagnosis is used:

A
  • for a minority of bacterial infections when organism is difficult or impossible to culture

Serodiagnosis: a diagnosis involving tests on blood serum or other serous fluid of the body. (E.g. identifying IgG/IgM levels, antibody levels, antigen levels, immunofluorescence)

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15
Q

Pros and cons of PCR:

A

Pros: sensitive & specific
Cons: prone to contamination by DNA, limited to targeted pathogen, test inhibited by substances in specimen

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16
Q

Steps for Gram Staining

A
  1. Bacteria are fixed to glass slide
  2. Apply crystal violet + wash
  3. Apply Lugol’s Iodine + wash
  4. Decolourisation w ethanol (gram -ve cells lose the gram complex but gram +ve cells retain it)
    - gram +ve appear purple
  5. Apply Saffranin counterstain + wash + dry
    - gram -ve coloured by counterstain => appear red
  6. Examine under oil immersion (w x100 lens)
17
Q

Which bacteria does Gram stain not work on:

A
  1. Too thin: treponema pallidum
  2. Dont retain stains: mycoplasma spp
  3. Dont let any stains in: mycobacterium spp
18
Q

What does MALDI-TOF detect?

A

Protein & peptides

19
Q

MacConkey agar is used for:

A

Test gram -ve bacteria

  • cuz it inhibits growth of gram +ve bacteria
  • lactose fermenters turn agar pink (due pH change)
    e.g. E.coli
20
Q

Gram stain: what step differentiates bacteria w a thick and thin peptidoglycan cell wall?

A

Decolourisation using acetone and alcohol