Isolamento di cellule T CD4 + da Linfonodi mouse utilizzando Miltenyi Purificazione MACS

Comment: Typo in water lysis portion of the protocol. Font for microliters translated as mL instead of uL. Use 900 uL of ddH20 and 100 uL of 10x PBS.

Thank you Melanie. That was a great presentation as we are trying to remove axillary lymph nodes and isolate T-cells for our experiments. Do you know by any chance what is an approximate number of cells (total vs T-cells (CD4+ and CD8+, etc)) can you isolate from axillary lymph from naive, let's say C57 or balb/c mice? We might need about, in best case scenario, at least 5*10^6. I appreciate any help you might provide us with. Good luck!

Sincerely,

Vyachesalv Palchevskiy

Hi, glad you found this video to be helpful. If you are only taking the axillary nodes and purifying naive cells I would use 3-4 mice to be sure you obtain the 5x10^6 that you need for CD4+ T cells. I would start with 4 since axillary nodes can vary in size. Typically the CD4 to CD8 ratio in a mouse is 2:1, though this varies between animals. If you need more lymph nodes from this region I suggest also taking the brachial nodes which are just underneath the skin, next to the muscle just below the fore'arm' of the mouse, number 5 on this chart: http://www.geocities.com/virtualbiology/lymph2.html I hope this helps and best of luck in all of your research!

Thank you. Do you ever digest lymph nodes or spleens to get dendritic cells? For us, looks like it affects viability and changes our FACS profile.

Thanks,

Vyacheslav Palchevskiy, Ph.D.

Hello! Thank you for the response (and the excellent answers that have followed). In our hands we have similar results where collagenase digestion reduces cell viability. We obtain more than enough dendritic cells from our single cell suspensions, therefore we avoid using collagenase. It may be particullarly useful in harvesting DCs from more collagen rich tissues (skin etc.).

Best wishes,

Melanie

Dear forum participants

I just wanted to comment on the subject of viability of cells after preparation with or without digestion. When following our general protocol for preparation of lymphoid organs without digestions (see our website), one can expect a viability of 90-95% for spleen. When doing a Collagenase digestion for the preparation of dendritic cells, as it is recommended for most of our murine dendritic cell products (e.g. CD11c MicroBeads), a very similar viability rate can be expected. Meaning, we do not observe a considerable difference in viability between digested and non-digested spleen tissue. The advantage of using Collagenase for dendritic cell isolations is, that one receives a higher yield of these rare target cells.

I hope this information was helpful for you.

Best regards,

Frank Hardung

- Technical Support –

Miltenyi Biotec GmbH

).  In the spleen we noticed if we digest with collagonase A + Dnase it decreases the flow for CD4 CD8 CD44 for example as compared to an undigested spleen - which digest do you recommend and what is the best way to talk with you or someone in your Co.

http://www.youtube.com/watch?v=aaqTUIFsdd0

Well- you seem to have enough time to make funny videos,...-
Anyway- if you would use the columns the right way (as described in detail in the datasheet) and if you would use a good cell suspension- you can quickly isolate your desired cells. I never had this problem before- it is fast and always works. Never had something as reliable as MACS beads in the lab!

How many T cells do you get out of a lymph node, or out of all the lymph nodes of one mouse?