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科创生物:FITC anti-human CD8 Antibody-B.S.BIO.

科创生物 / 2020-12-12 22:37:23

Catalog# / Size  XG-AB200325T/50T/100T

 

Description

Species Reactivity

Human

Clone

 1H12

Other Names

T8, Leu2

Isotype

Mouse IgG2b, κ

Description

CD8 (cluster of differentiation 8) is   a transmembrane glycoprotein that   serves as a co-receptor for the T cell   receptor (TCR). Like the TCR, CD8 binds to a major histocompatibility complex (MHC)   molecule, but is specific for the class I MHC protein. There   are two isoforms of the protein, alpha and beta, each encoded by a different   gene. In humans, both genes are located on chromosome   2 in position 2p12.The CD8 co-receptor is predominantly   expressed on the surface of cytotoxic T cells, but can also be found   on natural killer cells, cortical thymocytes,   and dendritic cells. It is expressed in T cell   lymphoblastic lymphoma and hypo-pigmented mycosis fungoides.

 

Product Details

Antibody Type

Monoclonal

Host Species

Mouse

Immunogen

Human CD8 Recombinant Protein

Formulation

Antibodies are supplied in buffer containing   stabilizer and 0.05%

sodium azide

Preparation

The antibody was purified by affinity   chromatography, and conjugated with FITC under optimal conditions.

Storage & Handling

Store protected   from light at 2-8°C. Do not freeze. The expiration date is indicated on the   vial label.

Application

FC - Quality tested

Recommended Usage

0.5ug/T

Excitation Laser

Blue Laser (488 nm)

LWB Cell Preparation

1.      For each patient   sample, label three  tubes A, B, and C.   Also label each tube with the sample identification number.

2.      Place 50 µL PBS   reagent into Tube A, Mouse IgG2b FITC Control reagent into Tube B, and 0.5ug of   the CD8-FITC reagent into Tube C.

3.      For each sample   tube, use a fresh micropipettor tip and carefully add 50 µL of human Peripheral   blood into the bottom of each of the three labeled tubes. All tubes refill to   100ul.

4.      Vortex thoroughly   at low speed for 3 seconds and incubate for 15minutes at room temperature (20°C–25°C).   Repeat this step again.

NOTE  Protect samples from direct light during this incubation procedure and   exercise care to prevent blood from running down the side of the tube. If   whole blood remains on the side of the tube, it will not be stained with the   reagent.

5.      Add 250uL of room   temperature (20°C–25°C)  lysing   solution to each tube. Immediately vortex thoroughly at low speed for 3   seconds and incubate for 10–

12 minutes at room temperature (20°C–25°C) in the   dark. Do not exceed 12 minutes.

6.      Immediately after   incubation, add 1 mL of PBS with 1% FBS to each tube. Centrifuge tubes at 1500rpm   for 5 minutes at room temperature (20°C–25°C).

7.      Aspirate the   supernatant leaving approximately 50 µL of residual fluid in the tube to   avoid disturbing the pellet.

8.      Repeat 6,7steps   again.

9.      Vortex thoroughly   at low speed to resuspend the cell pellet in the residual fluid and then add   0.3 mL of  PBS to each tube. Vortex   thoroughly at low speed for 3 seconds. Make sure the cells are well mixed   with the fixing solution.

10.    The cells are now   ready to be analyzed on the flow cytometer. Cap or cover the prepared tubes   and store at 2°C– 8°C in the dark until flow cytometric analysis.

NOTE  Analyze the fixed cells within 2 hours after staining.Over 2 hours add 0.3   mLof  PBS with 1% paraformaldehyde to   each tube.

 

Data

Flow Cytometry

 

Human peripheral   blood lymphocytes stained with CD8(1H12) FITC

 

For research use only. Not for diagnostic use. Not for resale. Suzhou Bright Scistar Biotech Co. Ltd will not be held responsible for patent infringement or other violations that may occur with the use of our products.

 

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