Purification of early-B-cell factor and characterization of its DNA-binding specificity.

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Mol Cell Biol. 1993 June; 13(6): 3392-3400

Purification of early-B-cell factor and characterization of its DNA-binding specificity.

A Travis, J Hagman, L Hwang and R Grosschedl

Howard Hughes Medical Institute, Department of Microbiology, University of California, San Francisco 94143-0414.

ABSTRACT

Early-B-cell factor (EBF) is a nuclear protein that recognizesa functionally important sequence in the promoter of the mb-1gene. Like the mb-1 gene, which encodes an immunoglobulin-associatedprotein, EBF is specifically expressed in the early stages ofB-lymphocyte differentiation. We purified EBF by sequence-specificDNA affinity chromatography and examined its biochemical propertiesand DNA-binding specificity. Crude nuclear extract and affinity-purifiedEBF generated protein-DNA complexes with the mb-1 promoter thatwere indistinguishable in electrophoretic mobility shift andDNase I footprint assays. Fractionation of affinity-purifiedEBF by sodium dodecyl sulfate-polyacrylamide gel electrophoresisand renaturation of isolated polypeptides indicated that EBFDNA-binding activity could be reconstituted from polypeptideswith molecular masses of 62 to 65 kDa. Gel filtration chromatographysuggested that native EBF has a molecular mass of 140 kDa, ifa globular shape of the protein is assumed. Thus, EBF appearsto be a dimer with subunits of 62 to 65 kDa. To characterizethe DNA-binding specificity of purified EBF, we performed twosets of experiments. First, we examined various mutant EBF-bindingsites for interaction with purified EBF in an electrophoreticmobility shift assay. Second, we used oligonucleotides containingpairs of randomized bases in a binding-site selection and amplificationexperiments to determine a preferred sequence for DNA bindingby EBF. Taken together, the results of these experiments indicatedthat EBF recognizes variations on the palindromic sequence 5'-ATTCCCNNGGGAAT,with an optimal spacer of 2 bp between the half-sites.

Mol Cell Biol. 1993 June; 13(6): 3392-3400

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