Cloning and functional analysis of the hematopoietic cell-specific phospholipase C(gamma)2 promoter.

Abstract:

:Phospholipase C(gamma)2 (PLCgamma2) is a phospholipid-converting enzyme which, upon receptor stimulation, is activated within membrane-bound signalling complexes. In contrast to the highly ubiquitous PLCgamma1, PLCgamma2 is expressed predominantly in B-lymphocytes. Associated with antigen-coupling receptors it is activated by tyrosine phosphorylation after the triggering of B-cell surface immunoglobulin. We have cloned and sequenced the human PLCgamma2 promoter. Primer extension analysis reveals the existence of a major transcriptional start site. The TATA-less promoter contains G+C-rich stretches with a cluster of contiguous SP1 consensus sites, an NF1, and an AP2 site between bp -220 to -70. A construct containing the region from -189 to +78 confers full promoter activity, as shown by fusion to a luciferase reporter gene construct. The distal part of the promoter between bp -662 to -293 containing an SRE, EBF and CACCC box contributed negatively to promoter activity in the B-cell line Raji but not in three adherent cell lines. In Raji cells, PLCgamma2 mRNA is expressed at low levels with a half life greater than 4 h. After treatment with serum, TPA, retinoic acid, or with 5-azacytidine increased levels of PLCgamma2 mRNA were induced in B-cells.

journal_name

FEBS Lett

journal_title

FEBS letters

authors

Kang JS,Kohlhuber F,Hug H,Marmé D,Eick D,Ueffing M

doi

10.1016/s0014-5793(96)01276-8

subject

Has Abstract

pub_date

1996-12-09 00:00:00

pages

14-20

issue

1-2

eissn

0014-5793

issn

1873-3468

pii

S0014-5793(96)01276-8

journal_volume

399

pub_type

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