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A complex composed of at least two HeLa nuclear proteins protects preferentially one DNA strand of the simple (gt) n (ga) m containing region of intron 2 in HLA ‐ DRB ‐genes
Author(s) -
Mäueler Winfried,
Frank Gabi,
Muller Marc,
Epplen Jörg T.
Publication year - 1994
Publication title -
journal of cellular biochemistry
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 1.028
H-Index - 165
eISSN - 1097-4644
pISSN - 0730-2312
DOI - 10.1002/jcb.240560112
Subject(s) - dna , intron , dna binding protein , electrophoresis , electrophoretic mobility shift assay , biology , biochemistry , nuclear protein , biophysics , hela , function (biology) , microbiology and biotechnology , chemistry , gene , in vitro , gene expression , genetics , transcription factor
Electrophoretic mobility shift assays reveal that HeLa neuclear proteins bind fast and with measurable affinity to target DNAs containing mixed simple repetitive (gt) n (ga) m stretches. Preincubation of the proteins at elevated temperature prevents the formation of the major DNA/protein complex in favour of several distinct assemblies. A similar pattern of retarded bands was observed employing higher salt concentrations in binding reaction. Thus conformational changes of different proteins appear to influence the complex rather than alternating DNA structures. Separation of the total nuclear extract into a water soluble and an insoluble protein fraction leads to a complete loss of target DNA bindinlg capability of the fractions. The binding capacity is restored by combining the two fractions suggesting that at least two protein components are necessary to form a complex with the target sequence. The proteins can be differentiated into head sensitive, water soluble and temporary stable, water insoluble, respectively. Furthermore, specifically binding polypeptides are not detectable by Southwestern analyses, probably because the essential components are separated during electrophoresis. DNase 1 footpoint analyses yield four different protein binding regions only on the (gt) n (ga) m harbouring strand. The footprints cover larger portions of the mixed simple repeat in addition to a portion 5′ of the (gt) n part. Hence at lealst two nuclear protein components of unknown biological function have to be present simultaneously to protect preferentially the (gt) n (ga) m ‐containing strand intron 2 in HLA‐DRB genes

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