A RAPID AND SIMPLE MICROFLUOROMETRIC PHAGOCYTOSIS ASSAY

被引：151

作者：

WAN, CP ^{[1
]}

PARK, CS ^{[1
]}

LAU, BHS ^{[1
]}

机构：

[1] LOMA LINDA UNIV,SCH MED,DEPT MICROBIOL,LOMA LINDA,CA 92350

来源：

JOURNAL OF IMMUNOLOGICAL METHODS | 1993年 / 162卷 / 01期

关键词：

PHAGOCYTOSIS; FLUORESCENCE ASSAY; FLUORESCEIN; J774-CELL; MICROPLATE FLUOROMETER;

D O I：

10.1016/0022-1759(93)90400-2

中图分类号：

Q5 [生物化学];

学科分类号：

071010 ; 081704 ;

摘要：

A microfluorometric method for phagocytosis study has been developed using fluorescein conjugated Escherichia coli K-12 particles. This technique is based on the uptake of fluorescent particles and quenching of extracellular fluorescence at the end of the assay. A murine macrophage cell line, J774, was used as a phagocyte model. The cells were harvested from tissue culture flasks and adjusted to 1 x 10(6) cells/ml. They were then dispensed into a 96-well tissue culture plate, 100 mul/well, and incubated at 37-degrees-C in 5% CO2 for 1 h to allow cells to adhere to the bottom of the wells. The culture medium was aspirated and 100 mul of fluorescent E. coli particles suspended in Hanks' buffer were added. The plates were further incubated for various time periods. Buffer solution in the wells was removed by aspiration. Extracellular fluorescence was then quenched by adding 100 mul of trypan blue (250 mug/ml, pH 4.4). The dye was removed after 1 min. The intensity of fluorescence associated with intracellular fluorescent particles was measured directly in the wells using a computerized microplate fluorometer at 485 nm excitation and 530 nm emission. This assay provided a rapid and objective measurement of phagocytosis activity. Using a cultured cell line and a 96-well microtiter plate format, this assay can facilitate the screening of a large number of various biological and pharmacological substances for their modulating effects on phagocytosis.

引用

页码：1 / 7

页数：7

共 30 条

[1] A RAPID RADIOMETRIC ASSAY FOR MEASURING PHAGOCYTOSIS OF SACCHAROMYCES-CEREVISIAE IN MACROPHAGE CULTURES [J].

BECKER, J ;

CARTER, SW ;

GRASSO, RJ .

JOURNAL OF IMMUNOLOGICAL METHODS, 1986, 91 (01) :1-10

[2] A FLUOROMETRIC ASSAY TO MONITOR MITOGENIC STIMULATION OF HUMAN-LYMPHOCYTES [J].

BIALEK, R ;

ABKEN, H .

JOURNAL OF IMMUNOLOGICAL METHODS, 1991, 144 (02) :223-229

[3] AUTOMATED FLUOROMETRIC ASSAY FOR T-CELL CYTO-TOXICITY [J].

BRENAN, M ;

PARISH, CR .

JOURNAL OF IMMUNOLOGICAL METHODS, 1988, 112 (01) :121-131

[4] ASSESSMENT OF PHAGOCYTIC-ACTIVITY OF GRANULOCYTES USING LASER FLOW-CYTOMETRY [J].

BUSCHMANN, H ;

WINTER, M .

JOURNAL OF IMMUNOLOGICAL METHODS, 1989, 124 (02) :231-234

[5] STAPHYLOCOCCUS-AUREUS PHAGOCYTOSIS - A NEW CYTOFLUOROMETRIC METHOD USING FITC AND PARAFORMALDEHYDE [J].

CANTINIEAUX, B ;

HARIGA, C ;

COURTOY, P ;

HUPIN, J ;

FONDU, P .

JOURNAL OF IMMUNOLOGICAL METHODS, 1989, 121 (02) :203-208

[6] MACROPHAGE PHAGOCYTOSIS - USE OF FLUORESCENCE MICROSCOPY TO DISTINGUISH BETWEEN EXTRACELLULAR AND INTRACELLULAR BACTERIA [J].

DREVETS, DA ;

CAMPBELL, PA .

JOURNAL OF IMMUNOLOGICAL METHODS, 1991, 142 (01) :31-38

[7] LYMPHOKINE-STIMULATED MACROPHAGE PHAGOCYTOSIS OF FLUORESCENT MICROSPHERES - A RAPID NEW ASSAY [J].

DUNN, PA ;

EATON, WR ;

LOPATIN, ED ;

MCENTIRE, JE ;

PAPERMASTER, BW .

JOURNAL OF IMMUNOLOGICAL METHODS, 1983, 64 (1-2) :71-83

[8]

ESSIGMARCELLO JS, 1990, IN VITRO TOXICOL, V3, P219

[9] SIMULTANEOUS MEASUREMENT BY FLOW-CYTOMETRY OF PHAGOCYTOSIS AND HYDROGEN-PEROXIDE PRODUCTION OF NEUTROPHILS IN WHOLE-BLOOD [J].

HASUI, M ;

HIRABAYASHI, Y ;

KOBAYASHI, Y .

JOURNAL OF IMMUNOLOGICAL METHODS, 1989, 117 (01) :53-58

[10] THE USE OF FLUORESCENCE QUENCHING IN FLOW CYTOFLUOROMETRY TO MEASURE THE ATTACHMENT AND INGESTION PHASES IN PHAGOCYTOSIS IN PERIPHERAL-BLOOD WITHOUT PRIOR CELL-SEPARATION [J].

HED, J ;

HALLDEN, G ;

JOHANSSON, SGO ;

LARSSON, P .

JOURNAL OF IMMUNOLOGICAL METHODS, 1987, 101 (01) :119-125

← 1 2 3 →