Immunologic Assay Flashcards
what are the parts of an immunoglobulin?
heavy chain and a light chain
variable region and constant region of each chain
which probes can immunoglobulin molecules be conjugated with?
- Fluorescence dyes for immunofluorescence (IF) staining
- Gold particles for immunoelectron microscopy
- Enzymes for immunohistochemistry, ELISA
the different probes are depending on the purpose
probes are usually conjugated to the contact region of immunoglobulin to preserve the antigen-binding property of the antibody
what is the purpose of direct IF assay?
to visualize the localization of antigen “X”, anti-X antibody is conjugated with FITC
it’s to study the localization of something in the cell
what is a cryostat section?
thin (6-10 mm) sections sliced from frozen tissue samples
many antibodies do not recognize the antigens in formalin-fixed samples due to conformational changes caused by fixation
cryostat sections are, thus, most frequently used for IF staining
what are the steps in doing a direct IF assay?
- cryostat sections are prepared from the tissue of interest
- ehe sections are incubated with FITC-conjugated antibody
- the antibody binds to antigen X expressed Cell Type A
- the sections are washed to remove unbound antibody
- the sections are observed under fluorescence microscope to visualize FITC-associated fluorescence signals
- antigen X can be visualized with green fluorescence
what does EBS stand for?
epidermolysis bullosa simplex
really nasty skin blisters
what mutation leads to EBS?
mutation of the keratin 5 or keratin 14 gene
specifically, a homologous one base pair deletion in exon 1
this mutation results in a frame shift and a formation of a premature termination codon
which test would help diagnose EBS?
IF staining
if you stain the tissue with anti-keratin 5 or anti-keratin 14 it would let you see if both proteins are present
if they’re present, they will show up bright green but if there’s no green showing up in the stain, you know the proteins are absent
how does immunoelectron microscopy work?
- an antibody against MHC class II molecule is labeled with gold particles, which appear as electron dense zones at the EM level
- ultra-thin skin sections are incubated with gold particle-labeled anti-MHC class II antibody.
- gold particles are found predominantly within multivesicular bodies, known as the MHC class II compartment (MIIC), where antigen processing and loading take place
what findings would support a SLE diagnosis?
- H&E staining of kidney biopsy shows a wire-loop lesion of glomerulus
- IF staining with FITC-conjugated anti-human IgG antibody reveals IgG deposition along glomerular capillary loops
- IF staining with FITC-conjugated anti-human C3 antibody reveals complement deposition as well
these changes indicate deposition of immune complex (IC) along glomerular capillary loops
how does immunohistomchemistry work?
it’s a modified version of IF staining!
an antibody is conjugated with an enzyme that converts a colorless substrate into a colored product
peroxidase and alkaline phosphatase are most commonly used to label the antibodies for this application
what kind of tissues can you do immunohistochemistry on?
although IF staining can be performed only with cryostat sections prepared from frozen tissues, immunohistochemistry may be applicable to conventional formalin-fixed tissues
what would a kidney biopsy of an SLE patient show?
IgG deposition along glomerular capillary loops
what’s the different between direct and indirect IF staining?
indirect IF staining enables the detection of auto-antibodies in SERUM samples
direct IF staining enables the detection of deposition of auto-antibodies in TISSUE biopsy samples = skin, kidney, etc.
how does indirect IF staining work?
a serum sample from an SLE patient can be tested for anti-nuclear antibody (ANA)
- human epithelial cell line (HEp-2) is incubated with serum to allow binding of ANA to the nuclei
- the cells are then incubated with FITC-conjugated anti-human IgG to allow the detection of ANA
- the IF image (green color) indicates the presence of ANA in the blood circulation
- the cells are counter-stained to indicate cytoplasmic areas (red color)
how can you estimate the relative antibody concentration in a serum sample?
by diluting a serum sample, one can estimate relative antibody concentration
- serum from an SLE patient is serially diluted and then tested for ANA
- if ANA is still detectable at 1:320 dilution and becomes undetectable at 1:640, it means the titer of 1:320
antibody titers are often used to follow the disease activity – a change from 1:40 to 1:160, for example, indicates an increase in circulating ANA concentration and, thus, implies exacerbation of the disease
by contrast, a change from 1:640 to 1:160 indicates a reduction in ANA concentration and, thus, implies improvement of the disease
what do different staining patterns in indirect IF staining mean?
different staining patterns imply different distributions of antigens recognized by autoantibodies
ex. the auto-antigen recognized in one person could be located at the inter-cellular space between keratinocytes while another person may have auto-antigen recognized at the basement membrane and they would be two totally different diseases!
pemphigus vulgaris vs. bullous pemphigoid
what are the steps in a Western blot?
it analyzes the biochemical properties of an antigen
- tissue and cell extracts containing antigens are separated by SDS-PAGE based on the molecular weight
- the proteins are transferred to a membrane
- he membrane is incubated with a serum sample containing antibodies
- he membrane is then incubated with enzyme-conjugated anti-IgG
- he membrane is developed by addition of colorless substrate
- colored band indicates the location (molecular weight ) of the antigen
what is an example of a diagnostic application of immunoblotting? aka Western Blot
- Human keratinocyte extracts are separated in SDS-PAGE
- proteins are transferred onto a membrane
- the membrane is stained with Coomassie blue for all proteins
- the membrane is incubated with serum from Pt #1 (Pemphigus vulgaris), a new patient, or healthy volunteer
- a band of about 130 kD (desmoglein-3) is detected with serum samples from Pt #1 and the new patient
- the results imply that auto-antibodies in both patients recognize an antigen of the same molecular size
what are the steps in an ELISA?
- Test samples containing antigen “X” (red triangles) are immobilized to the bottoms of a 96-well plate
- enzyme-conjugated anti-X antibody is added to the plate
- colorless substrate is added to the plate
- development of colored products indicates the presence of antigen X in the test samples
it’s those plates with a ton of holes you used to use to calibrate purple with in Sakima’s lab
what is an ELISA used for?
- to measure the amount of antigen
2. to measure the amount of antibodies
how is an ELISA used to measure the amount of antigen?
- to test the concentration of IL-1 in human serum samples, anti-IL-1 monoclonal antibody (produced in mice) is first immobilized onto the 96 well plate
- graded amounts of recombinant IL-1 are added to individual wells to create a standard curve – IL-1 molecules (red triangles) are captured by anti-IL-1 antibody
3 .serum samples are also added to individual wells
- nzyme-conjugated anti-IL-1 monoclonal antibody (which binds to a different epitope) is added to the plate
- colorless substrate is then added to the plate
- the amount of IL-1 in a test sample can now be calculated from the standard curve
how can an ELISA be used to measure the amount of antibodies?
- to test the concentration of antibody against demoglein-3, recombinant desmoglein-3 proteins (red triangles) are immobilized onto a 96 well plate.
- serum samples from pemphigus vulgaris patients are added to individual wells
- enzyme-conjugated anti-human IgG is added to the plate
- colorless substrate is then added to the plate
- one can estimate the amount of anti-desmoglein-3 antibody in the sample based on the standard curve
what is an agglutination test used for?
- it enables rapid detection of antigen-reactive antibodies
2. also enables rapid detection of antigens
