1-10 Flashcards

1
Q

Negative agglutination:

A
  • Solid “button” sediment with turbid supernatant
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2
Q

Name two types of haemagglutination tests

A
  • Direct haemagglutination: detect antibodies against red cell determinants - Passive haemag.: …against compounds artificially coupled to red cells
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3
Q

The essential differences between agglutination and precipitation are in:

A
  • size, solubility and location of the antigen - in agglutination the antigens are whole cells, like red cells but in precipitation the antigen is a soluble molecule
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4
Q

Radial immunodiffuion (RID)

A

is quantitative method used for quantification

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5
Q

Immunoelectrophoresis (IEF)

A

precipitation reaction, in which direct current is used to regulate the movement of antigen and antibody molecules in agar or agarosis gel

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6
Q

Seperation of proteins in electric field depends on:

A
  • Whole electric charge - Molecular mass - Isoelectric point
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7
Q

Serum proteins separate into six major fractions according to their charge at given pH

A
  • α1-globulins, α2-globulins, β-globulins, γ-globulins, hydragel protein K20, hydragel proteins (E)
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8
Q

What does ELISA stand for?

A
  • Enzyme-Linked ImmunoSorbent Assay - Result: soluble colour product
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9
Q

Application of EIA can be used for:

A
  • Qualitative detection of the presence of Ab or Ag - Quantitative determination concentration of Ab or Ag
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10
Q

Advantage of EIA:

A
  • Detection of Ag of pathogens directly - Detection of Ab against many bacterial, viral or parasitic agents - Very flexible method
    Disadvantage: false positive results
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11
Q

ELISA techniques are divided to what two groups?

A
  • For detection of antigens: sandwich ELISA & competitive ELISA - For detection of antibodies: direct ELISA & blocking ELISA
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12
Q

Name two different types of IFA

A
  • Direct immunofluorescence staining - the primary Ab is labelled with fluorescence dye - Indirect immunofluorescence staining - secondary reagent (antiglobulin or protein A/G labelled with fluorophore) is used to recognize a primary Ab - Advantages: identification of antigenic structures, identif. of different antigens in one sample, identif. of the live and dead bacteria in one sample, rapid method
  • Disadvantages: requirement of expensive equipment and reagents and trained personnel Green fluorescence - live cells Red fluorescence - dead cells
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