A STANDARDIZED PROTOCOL FOR FLOW CYTOMETRIC ANALYSIS OF CELLS ISOLATED FROM CEREBROSPINAL-FLUID

被引：60

作者：

DUX, R

KINDLERROHRBORN, A

ANNAS, M

FAUSTMANN, P

LENNARTZ, K

ZIMMERMANN, CW

机构：

[1] UNIV ESSEN GESAMTHSCH,DEPT NEUROL,D-45147 ESSEN,GERMANY

[2] UNIV ESSEN GESAMTHSCH,INST CELL BIOL CANCER RES,D-45147 ESSEN,GERMANY

来源：

JOURNAL OF THE NEUROLOGICAL SCIENCES | 1994年 / 121卷 / 01期

关键词：

FLOW CYTOMETRY; CEREBROSPINAL FLUID; MONOCLONAL ANTIBODIES; MALIGNANT CELLS;

D O I：

10.1016/0022-510X(94)90159-7

中图分类号：

R74 [神经病学与精神病学];

学科分类号：

摘要：

Flow cytometry (FC) is an useful tool for the analysis of subpopulations in complex cell suspensions. When applying this method to the cerebrospinal fluid (CSF), some characteristic properties of this cell type must be taken into consideration: there are only few cells which decay rapidly in their native medium and during centrifugation. One aim of the immunostaining procedure preceding flow cytometric analysis must be to minimize cell loss in order to get an undistorted picture of 'true' CSF cell populations. Consequently, morphological flow cytometric plots of high resolution are an indispensable precondition for reliable determination of subpopulations defined by monoclonal antibody (Mab) binding. We describe a standardized protocol for the flow cytometric examination of CSF cells which minimizes undesired cell loss. By the use of a 'quality control' the extent of cell loss could be monitored. Examples of morphological flow cytometric plots are given. The subsequent determination of Mab binding subpopulations is critical when fluorescence intensities of antigen positive and negative cells are non-disjunct. A statistical test was developed for these cases often seen when cell surface determinants are expressed at low levels only.

引用

页码：74 / 78

页数：5

共 15 条

[1] AHRENS O, 1980, FLOW CYTOMETRY, V4, P112
[2] ACUTE MULTIPLE-SCLEROSIS EXACERBATIONS ARE CHARACTERIZED BY LOW CEREBROSPINAL-FLUID SUPPRESSOR CYTOTOXIC T-CELLS
ANTONEN, J
SYRJALA, P
OIKARINEN, R
FREY, H
KROHN, K
[J]. ACTA NEUROLOGICA SCANDINAVICA, 1987, 75 (02): : 156 - 160
[3] MONOCLONAL ANTIBODY-DEFINED IMMUNOREGULATORY CELLS IN MULTIPLE-SCLEROSIS CEREBROSPINAL-FLUID
CASHMAN, N
MARTIN, C
EIZENBAUM, JF
DEGOS, JD
BACH, MA
[J]. JOURNAL OF CLINICAL INVESTIGATION, 1982, 70 (02) : 387 - 392
[4] CALIBRATION OF FLUORESCENCE INTENSITIES TO QUANTIFY ANTIBODY-BINDING SURFACE DETERMINANTS OF CELL SUBPOPULATIONS BY FLOW-CYTOMETRY
DUX, R
KINDLERROHRBORN, A
LENNARTZ, K
RAJEWSKY, MF
[J]. CYTOMETRY, 1991, 12 (05): : 422 - 428
[5] INCREASED PROPORTION OF CD4+CDW29+CD45R-UCHL-1+ LYMPHOCYTES IN THE CEREBROSPINAL-FLUID OF BOTH MULTIPLE-SCLEROSIS PATIENTS AND HEALTHY-INDIVIDUALS
HEDLUND, G
SANDBERGWOLLHEIM, M
SJOGREN, HO
[J]. CELLULAR IMMUNOLOGY, 1989, 118 (02) : 406 - 412
[6] KINDLERROHRBORN A, 1985, DIFFERENTIATION, V30, P65
[7] PARAFORMALDEHYDE FIXATION OF HEMATOPOIETIC-CELLS FOR QUANTITATIVE FLOW-CYTOMETRY (FACS) ANALYSIS
LANIER, LL
WARNER, NL
[J]. JOURNAL OF IMMUNOLOGICAL METHODS, 1981, 47 (01) : 25 - 30
[8] FLOW-CYTOMETRY AS AN ANALYTICAL AND PREPARATIVE TOOL IN IMMUNOLOGY
LOKEN, MR
STALL, AM
[J]. JOURNAL OF IMMUNOLOGICAL METHODS, 1982, 50 (03) : R85 - R112
[9] THE IMBALANCE IN CSF T-CELL SUBSETS IN ACTIVE MULTIPLE-SCLEROSIS
MATSUI, M
MORI, KJ
SAIDA, T
AKIGUCHI, I
KAMEYAMA, M
[J]. ACTA NEUROLOGICA SCANDINAVICA, 1988, 77 (03): : 202 - 209
[10] MIX E, 1990, CLIN EXP IMMUNOL, V79, P21

← 1 2 →