Flow-cloned cells

• Next message: Akos_Szilvasi@biogen.com: "Re: problems with time delay calibration on FACS Calibur"
• Previous message: Tom Mc Closkey: "Re: Isolation of kupffer cells"
• Next in thread: Mario Roederer: "Re: Flow-cloned cells"
• Reply: Mario Roederer: "Re: Flow-cloned cells"
• Maybe reply: Shari_Brezinsky@biogen.com: "Re: Flow-cloned cells"
• Messages sorted by: [ date ] [ thread ] [ subject ] [ author ]

Hi,

For those who have experience cloning cells, what do you do to insure that
single cells, cloned by FACS into 96-well plates, continue to grow?  Add
factors (if so, which) or cell growth-conditioned medium?  Although any
suggestions in general will be appreciated, the cells in question at the
moment are 293 cells (human kidney carcinoma, I believe).  Any advice would
be appreciated.

Thanks.

Ray

Raymond B. Hester, Ph.D.
Research Cytometry Laboratory
CSAB 357, Biotechnical Services
University of South Alabama
Mobile, AL 36688
Voice:	  (334) 460-6029
FAX:	  (334) 460-6073
E-mail:   rhester@jaguar1.usouthal.edu

• application/ms-tnef attachment: winmail.dat

• Next message: Akos_Szilvasi@biogen.com: "Re: problems with time delay calibration on FACS Calibur"
• Previous message: Tom Mc Closkey: "Re: Isolation of kupffer cells"
• Next in thread: Mario Roederer: "Re: Flow-cloned cells"
• Reply: Mario Roederer: "Re: Flow-cloned cells"
• Maybe reply: Shari_Brezinsky@biogen.com: "Re: Flow-cloned cells"
• Messages sorted by: [ date ] [ thread ] [ subject ] [ author ]

This archive was generated by hypermail 2b29 : Sat Mar 10 2001 - 19:31:24 EST