Specimen Nr. 04B

Specimen:

Spleen (Rat), subpopulations of B lymphocytes

Staining:

Peroxidase, anti-peroxidase technique, nucleus stained with hemalaun

Magnification:

80x

Important structures :

1.Marginal zone of white pulp
2.Primary lymphoid follicle
3.Central artery
4.Periarteriolar lymphoid sheath (PALS)
5.Red pulp
Mit einem Antikörper sind immunhistochemisch in braun B-Lymphozyten dargestellt. Sie befinden sich in der Hauptsache in den Follikeln und der Marginalzone. Aber auch in der roten Pulpa und der PALS werden B-Lymphozyten gefunden. Neben den B-Lymphozyten befinden sich in der roten Pulpa auch noch viele Plasmazellen.

Legende:

Marginal zone of white pulp
Primary lymphoid follicle
Central artery
Periarteriolar lymphoid sheath (PALS)
Red pulp

Localisation of organs of immune-lymphatic system[we]

1. Pharyngeal tonsil
2. Palatine tonsil
3. Lymph node
4. Lymphatic vessels
5. Spleen
6. Peyer's patches
7. Thymus

Immunohistochemestry

Immunohistochemistry is used to confirm the presence of or to identify certain structures or substances in tissue sections which cannot be identified with conventional staining methods. Such structures include: cells, enzymes, hormones, macromolecules like nucleic acids and polysaccharides. The basis of immunohistochemical staining techniques is the antigen-antibody reaction. This method makes it possible to differentiate, for example, various cells in a tissue section according to their different metabolic products or surfaces. Either the metabolic product or a certain surface component serves as the antigen. In the first step, the antigen reacts with a specific antibody. The resulting antigen-antibody complex is invisible. Therefore, in a further step a second antibody bound to an adjuvant is added and binds to the initial antibody (so-called sandwich procedure). The bound adjuvant makes the antigen-antibody complex visible under the microscope and identifies the sought structure. Adjuvants are:

Combination with further dyes or staining techniques:

B-Lymphozyten gelangen über die Gefäße der Marginalzone in die Milz und verlassen sie nach einigen Stunden. Wenn B-Lymphozyten allerdings bei ihrer Wanderung durch die PALS auf einen aktivierten T-Lymphozyten gleicher Antigenspezifität treffen, induzieren jeweils 1-3 B-Lymphozyten einen Sekundärfollikel. Dort vermehren sich die antigen-spezifischen B-Lymphozyten und erhöhen die Affinität ihres Rezeptors. Auf diese Weise entstehen Plasmazellen, die sofort Antikörper produzieren (humorale Immunantwort), und Gedächtnis B-Lymphozyten, die im Vergleich zu nativen B-Lymphozyten bei einem zweiten Treffen mit demselben Antigen schneller größere Mengen Antikörper produzieren.
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Magnification:

80x

Magnification:

80x

Magnification:

80x

Magnification:

150x

Magnifications
Marginal zone of white pulp
Marginal zone of white pulp
Primary lymphoid follicle
Primary lymphoid follicle
Central artery
Central artery
Periarteriolar lymphoid sheath (PALS)
Periarteriolar lymphoid sheath (PALS)
Red pulp
Red pulp
Red pulp

HistoNet2000 - Help

1. Organization of the screen surface

Right side: histologic specimen
Left side: information about the specimen (above) and general program functions (below)

2.Histologic specimen

Pull the mouse across the histologic specimen for training purposes. A small square with exclamation marks (dynamic labels) will appear where there is an important structure. You should then decide what structure this could be. To check your result, simply click the appropriate square, and the correct label will appear. The option “marked” allows you to see all labels for all structures simultaneously. These can be removed by clicking “unmarked”. This reactivates the dynamic labels.

3. Complementary information

Info: general information about the specimen, as well as a list of the dynamic labels
Drawing: schematic drawing of the specimen
Staining: information about the staining method for this specimen
Knowledge: short texts with basic histologic information, presently deactivated

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