Diagnosis of Infection Flashcards

1
Q

What are the 2 ways that a pathogen can be identified?

A
  • identification of the actual pathogen
  • identification of the host response to the pathogen
  • ex. tuberculosis can be found in the lungs, or antibodies for tuberculosis can be found in serology
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2
Q

Which gene can be isolated that is known to cause methicillin resistance?

A

MECAG gene

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3
Q

What two pieces of information is important when identifying a microorganism?

A
  • presence of that microorganism

- susceptibility and the presence of a resistance gene

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4
Q

In what cases is it most useful to detect the specific antibodies to a pathogen rather than the actual pathogen?

A
  • pathogens that cannot be cultivated/ takes a long time to cultivate (tuberculosis is mostly identified via presence
  • high risk group pathogens
  • retrospective diagnosis
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5
Q

How does PCR work?

A

you design a primer that has a specific gene within the organism- you want to design a primer that is specific to the neisseria menigitis -> needs to be specific to the certain species – need to make primer that target specific resistance genes
- if you have a primer that targets a specific gene, you can determine methacillin resistance/specific

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6
Q

What are the advantages of non-culture methods?

A
  • fast
  • less labor intensive
  • suitable for organisms that cannot be cultured in the lab
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7
Q

What are some examples of non-culture methods?

A
  • microscopy
  • immunodiagnostics
  • molecular diagnostics
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8
Q

What is the main disadvantage of using an electron microscope?

A
  • cannot image live cells
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9
Q

What is resolution?

A
  • the minimum distance that you can distinguish two objects as two objects
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10
Q

What are the four steps of the gram stain?

A
  1. flood with crystal violet
  2. flood with iodine
  3. flood with ethanol
  4. flood with safarin
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11
Q

What piece of information does the gram stain give you?

A
  • tells you information about the structure of the cell wall of the pathogen
  • tells you the morphology of the bacteria (any stain will do this, but only the gram stain will tell you about the cell wall)
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12
Q

Acid fast cells are ______

A

very difficult to stain - cannot wash these cells with acid after they have been stained- if you do the organism will just retain the dye
- acid fast bacteria cannot retain the gram stain - if you cannot find the microorganism after doing a test then you will most likely have an acid fast bacteria

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13
Q

Describe florescent staining?

A
  • naturally florescent
  • stained with florescent dyes
  • many of the florescent methods empty antibodies that tag specific antigens on the cell surface- these antibodies are tagged with florescent materials
  • can use this method to detect even one cell in the specimen, because the signal is that strong
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14
Q

Describe electron microscopy

A

Gives a resolution of 0.1 to 1.0 nm

  • uses an electron beam instead of light
  • uses magnets instead of lenses to create an image
  • the specimen has to be very thin to work
  • shoes the surface of the organism opposed to the inside of the specimen
  • can show viruses even
  • not usually used in labs
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15
Q

In what cases is imumunodetection used?

A
  • used when you need a response much faster than you would get with just culturing
  • specific antibody coated onto a latex bead shows visible clumping
  • unusually used when bacterial meningitis is suspected - used with Strep pneumoniae, haemophilic influenzae, neisseria meningiditis in CSF
  • can sometimes lead to false positives
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16
Q

What does ELISA allow you to do?

A
  • allows you to quantify the pathogen, not just be able to tell if its present or not
  • the secondary antibodies that are produced are labeled with an enzyme
  • ALLOWS YOU TO TEST FOR ANTIBODIES FOR THE PATHOGEN
17
Q

How do you quantify ELISA?

A
  • can use spectrophotometry - more antibodies, more antibodies binding to more antigens and therefore there is more colour being produced
  • we would want this assay more than the other one because it allows us to use the same secondary antibodies to detect any human antibodies
18
Q

What is the process of using ELISA?

A
  • need to add the antigen to a test of the blood
  • if the antibody levels are high, the antibodies and antigen with agglutinate
  • if there is an secondary antibody complex, you can put a tag on it to detect the antibodies in the blood
  • tagging the secondary antibody is very critical- it will light it up
  • the secondary antibody will bind to the Fc region of the antigen
19
Q

What is ELISA quantified with?

A

can quantify this with a spectrophotometer which can quantify the intensity of the colour
- the more intense the colour, the more intense and severe the infection

20
Q

What does ELISA stand for?

A

Enzyme linked immunosorbent assay

21
Q

What are the 2 methods of detecting specific genes?

A
  • probe based methods (labeled, single stranded nucleic acid fragment to hybridize with the target DNA)
  • amplification based methods
22
Q

Culture based methods can be either ___ or ___ media

A

solid

liquid

23
Q

What is the culture based method of detecting obligate intracellular organisms?

A
  • very labour intensive and slow

- uses imumunodetection, molecular methods to detect

24
Q

What do biochemical tests entail?

A
  • they are based on what kinds of things organisms eat - gives you an idea of what kind of organism might be available in the specimen
  • these organisms can utilize glucose, lactose, maltose, etc