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specific immunodetection of cyclins using 488/630 dual laser flow cytometry

2019.4.26
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Phenotype-specific immunodetection of cyclins using 488/630 nm dual laser flow cytometry

William Telford 
Hospital for Special Surgery

This protocol is for use with the D and E cyclins and employs 488 nm argon laser excitation of propidium iodide and a FITC-conjugated phenotypic label, and 630 nm NeNe or diode laser excitation of the fluorochrome Cy5 to detect cell cycle-specific cyclin D expression. Unlike previously used below 0°C fixation protocols, this method employs a gentle ethanol fixation step, preserving surface marker expression and immunolabeling. It has been tested with antibodies against cyclin D1 (Pharmingen cat. no. 14561A, clone G12-4326), cyclin D2/D3 (cat. no. 14711A, clone G107-22) and cyclin E, and is based on protocols originally designed by Z. Darzynkiewicz. It can also be used with other cyclin antibodies (such as those against cyclin A and B1) and antibodies against proliferating cell nuclear antigen (PCNA) shown to be detectable with a single ethanol fixation step. This assay can be used with any instrument employing dual laser excitation, including the B-D Vantage, FACSCalibur and Coulter Elite.

 Materials

Procedure

 

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This technique has been used successfully to detect cyclin expression in several tumor cell lines, activated human lymphocytes and chick chondrocytes. Below, HL-60 cells labeled for cyclin D1 either with 80% EtOH treatment at –20°C or 70% EtOH at 4°C.ReferencesGong, J., Bhatia, U., Traganos, F. and Darzynkiewicz, Z. 1995. Expression of cyclins A, D2 and D3 in individual normal mitogen stimulated lymphocytes and in MOLT-4 leukemic cells analyzed by multiparameter flow cytometry. Leukemia 9, 893-899.

Juan G., Gong, J., Traganos, F. and Darzynkiewicz, Z. 1996. Unscheduled expression of cyclins D1 and D3 in human tumour cell lines. Cell Prolif. 29, 259-266 . 


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