Isolation of Untouched Human CD4+ T Cells from Peripheral Blood Mononuclear Cells (PBMC)

This product is intended for isolation of untouched human CD4⁺ T cells from peripheral blood mononuclear cells (PBMC) by depleting B cells, NK cells, monocytes, platelets, dendritic cells, CD8+ T cells, granulocytes and erythrocytes. Isolated CD4⁺ T cells are bead- and antibody-free and are suitable for any downstream application.

Principle of Isolation

A mixture of mouse IgG antibodies against the non-CD4⁺ T cells is added to the starting sample and allowed to bind to the cells. Depletion MyOne™ Dynabeads® are added and will bind to the antibodylabelled cells during a short incubation. The bead-bound cells are subsequently separated on a magnet and discarded. The remaining, untouched human CD4+ T cells can be used for any application


Downstream Applications

Isolated CD4+ T cells can be used in any application, e.g.:

• Studies on CD4⁺ T cell proliferation, apoptosis and induction of anergy
• Studies on antigen specific T cells
• Studies on regulation of CD4⁺ T cell cytokine expression
• Flow cytometry/FACS sorting

Sample Preparation

Untouched CD4+ T cells are isolated from a PBMC suspension. We recommend using a sample preparation procedur  that gives low platelet numbers. See Technical Recommendations, or visit Pan Mouse IgG - Depletion or Positive Isolation of Cells from Different Species for recommended sample preparation procedures.

Additional Materials Required

• Mixer allowing both tilting and rotation.
• Magnet: We recommend DynaMag™-15(cat.no. 123.01D) for 1-15 ml samples and DynaMag™-50 (cat.no. 123.02D) for 5-50 ml samples. Dynal® MPC™ magnets may also be used, except Dynal® MPC-1 (cat.no. 120.01D).
• Isolation buffer: Ca²⁺ and Mg²⁺ free phosphate buffered saline (PBS) (e.g. Gibco cat.no. 10010-023) supplemented with 0.1% BSA and 2mM EDTA.
• Heat inactivated Fetal Bovine Serum (FBS)/Fetal Calf Serum (FCS).
• Lymphoprep® for PBMC preparation (Axis Shield PoC, Norway).

Note:

• BSA can be replaced by human serum albumin (HSA) or 2% FBS/ FCS.
• EDTA can be replaced by 0.6% sodium citrate.
• PBS containing Ca²⁺ or Mg²⁺ is not recommended.

Critical notes

• Dynabeads® should be washed before use (see Dynabeads® Washing Procedure).
• Use a mixer that provides tilting and rotation of the tubes to ensure that Dynabeads® do not settle in the tube
• This product should not be used with Dynal® MPC™-1 (cat.no. 120.01D). See Technical Recommendations.
• Follow the recommended volumes and incubation times.
• Avoid air bubbles during pipetting.
• Keep the buffers cold!

1. Resuspend the Dynabeads® in the vial.


2. Transfer the desired volume of Dynabeads® to a tube.


3. Add the same volume of Isolation buffer, or at least 1 ml, and mix.


4. Place the tube in a magnet for 1 min and discard the supernatant.


5. Remove the tube from the magnet and resuspend the washed Dynabeads® in the same volume of Isolation buffer as the initial volume of Dynabeads® (step 2).

1. Transfer 100 μl (1 × 10⁷) PBMC in Isolation Buffer to a tube.


2. Add 20 μl heat inactivated FCS.


3. Add 20 μl of Antibody Mix.


4. Mix well and incubate for 20 min at 2-8°C.


5. Wash the cells by adding 2 ml Isolation Buffer. Mix well by tilting the tube several times and centrifuge at 300 × g for 8 min at 2-8°C. Discard the supernatant.


6. Resuspend the cells in 100 μl Isolation Buffer.


7. Add 100 μl pre-washed Depletion MyOne Dynabeads®.


8. Incubate for 15 min at 18-25°C with gentle tilting and rotation.


9. Resuspend the bead-bound cells by vigorously pipetting >10 times using a pipette with a narrow tip opening (e.g. a 1000 μl pipette tip or a 5 ml serological pipette).


10. Add 1 ml Isolation Buffer.


11. Place the tube in the magnet for 2 min.


12. Transfer the supernatant to a new tube.


13. Repeat step 10-12 with the tube containing the Dynabeads® and combine the two supernatants.

1. Dilute 10 - 15 ml buffy coat with PBS Isolation buffer to a total volume of 35 ml at 18-25°C (RT).


2. Add the diluted buffy coat on top of 15 ml of Lymphoprep®.


3. Centrifuge at 160 x g for 20 min at RT. Allow to decelerate without brakes.


4. Remove 18-20 ml of supernatant to eliminate platelets.


5. Centrifuge at 350 x g for 20 min at RT. Allow to decelerate without brakes.


6. Recover PBMC from the plasma/Lymphoprep® interface and transfer the cells to a 50 ml tube.


7. Wash PBMC once with Isolation buffer by centrifugation at 400 x g for 8 min at 2-8°C.


8. Wash PBMC twice with Isolation buffer by centrifugation at 225 x g for 8 min at 2-8°C and resuspend the PBMC at 1 x 10⁸ PBMC per ml in Isolation buffer.

1. Aasheim HC et al (2005) Ephrin-A1 binding to CD4+ T lymphocytes stimulates migration and induces tyrosine phosphorylation of PYK2. Blood 105: 2869-2876.


2. Jarnak-Jankovic S et all (2005) Evaluation of dendritic cells loaded with apoptotic cancer cells or expressing


3. tumour mRNA as potential cancer vaccines against leukemia. BMC Cancer. 5:20 doi:10.1186/1471-2407-5-20.


4. Zhang R et al (2004) CD40 ligand dysregulation in HIV infection: HIV glycoprotein 120 inhibits signalling cascades upstream of CD40 ligand transcription. J. Immunol. 172:2678-2686.


5. Hamez-Cognasse et al (2008). Direct contact of platelets and their released products exert different effects on human dendritic cell maturation. BMC Immunology 9:54 doi:10.1186/1471-2172-9-5.


6. Ghannam et al (2008). Human CD3 Deficiency Associated with Impairments in Dendritic Cell Differentiation, Memory B Cells, and Regulatory T Cells. The Journal of Immunology 184: 5158-5166.