Follicular dendritic cells mediated maintenance of primary lymphocyte cultures for long-term analysis of a functional in vitro immune system

被引:18
作者
Qin, DH
Wu, JH
Burton, GF
Szakal, AK
Tew, JG
机构
[1] Virginia Commonwealth Univ, Med Coll Virginia, Dept Microbiol & Immunol, Div Immunobiol, Richmond, VA 23298 USA
[2] Virginia Commonwealth Univ, Med Coll Virginia, Dept Anat, Div Immunobiol, Richmond, VA 23298 USA
来源
JOURNAL OF IMMUNOLOGICAL METHODS | 1999年 / 226卷 / 1-2期
关键词
follicular dendritic cell; primary lymphocyte culture; antibody; apoptosis; TUNEL;
D O I
10.1016/S0022-1759(99)00038-1
中图分类号
Q5 [生物化学];
学科分类号
071010 ; 081704 ;
摘要
Primary lymphocyte cultures are important for analysis of cellular and molecular events occurring during immune responses. However, the lymphoid cells (especially B cells) typically only survive for a few days in vitro which limits studies. Establishment of long-term primary lymphocyte cultures where a functioning humoral immune responses can be maintained and regulated is still a challenge. Follicular dendritic cells (FDC) are immune accessory cells that reside in the follicles of secondary lymphoid organs and are known to protect lymphocytes from apoptosis. We hypothesized that addition of FDC to primary lymphocyte cultures may help maintain humoral immune responses in vitro as they do in vivo. To test the hypothesis, freshly isolated lymphocytes were cultured with or without FDC. The B cells in cultures were labeled using B220 and apoptotic cells were labeled using the TUNEL assay. Antibody production was monitored in supernatant fluids using ELISA. The results showed that FDC reduced apoptosis and helped sustain primary lymphocyte cultures and antibody production was maintained throughout the entire period (e.g., 8 weeks). This FDC dependent system should be useful for analysis of cellular and molecular events over extended periods in vitro. (C) 1999 Elsevier Science B.V. All rights reserved.
引用
收藏
页码:19 / 27
页数:9
相关论文
共 19 条
[1]   F4-80, A MONOCLONAL-ANTIBODY DIRECTED SPECIFICALLY AGAINST THE MOUSE MACROPHAGE [J].
AUSTYN, JM ;
GORDON, S .
EUROPEAN JOURNAL OF IMMUNOLOGY, 1981, 11 (10) :805-815
[2]   MOLECULAR CONTROL OF B-LYMPHOCYTE GROWTH AND DIFFERENTIATION [J].
BANCHEREAU, J ;
BRIERE, F ;
LIU, YJ ;
ROUSSET, F .
STEM CELLS, 1994, 12 (03) :278-288
[3]  
BRITTON S, 1968, J IMMUNOL, V100, P1326
[4]  
BURTON GF, 1993, J IMMUNOL, V150, P31
[5]   REGULATION OF ANTIBODY FORMATION BY SERUM ANTIBODY .2. REMOVAL OF SPECIFIC ANTIBODY BY MEANS OF EXCHANGE TRANSFUSION [J].
BYSTRYN, JC ;
GRAF, MW ;
UHR, JW .
JOURNAL OF EXPERIMENTAL MEDICINE, 1970, 132 (06) :1279-&
[6]  
CAMPBELL DH, 1970, METHOD IMMUNOL, P246
[7]   INVITRO DEVELOPMENT OF LYMPHOCYTES-B FROM LONG-TERM CULTURED PRECURSOR CELLS [J].
DENIS, KA ;
WITTE, ON .
PROCEEDINGS OF THE NATIONAL ACADEMY OF SCIENCES OF THE UNITED STATES OF AMERICA, 1986, 83 (02) :441-445
[8]   IDENTIFICATION OF PROGRAMMED CELL-DEATH INSITU VIA SPECIFIC LABELING OF NUCLEAR-DNA FRAGMENTATION [J].
GAVRIELI, Y ;
SHERMAN, Y ;
BENSASSON, SA .
JOURNAL OF CELL BIOLOGY, 1992, 119 (03) :493-501
[9]   REGULATION OF ANTIBODY FORMATION BY SERUM ANTIBODY .I. REMOVAL OF SPECIFIC ANTIBODY BY MEANS OF IMMUNOADSORPTION [J].
GRAF, MW ;
UHR, JW .
JOURNAL OF EXPERIMENTAL MEDICINE, 1969, 130 (05) :1175-&
[10]   FOLLICULAR DENDRITIC CELLS AND THE MAINTENANCE OF IGE RESPONSES [J].
HELM, SLT ;
BURTON, GF ;
SZAKAL, AK ;
TEW, JG .
EUROPEAN JOURNAL OF IMMUNOLOGY, 1995, 25 (08) :2362-2369
12