HUMAN GENE FOR THE LARGE SUBUNIT OF RIBONUCLEOTIDE REDUCTASE (RRM1) - FUNCTIONAL-ANALYSIS OF THE PROMOTER

Parker, NJ; Begley, CG; Fox, RM

Author(s): Parker, NJ; Begley, CG; Fox, RM;
Details: Publication Year 1995-05-20,Volume 27,Issue #2,Page 280-285
Journal Title: GENOMICS
Publication Type: Journal Article
Abstract: Ribonucleotide reductase comprises two nonidentical protein subunits R1 and R2, both of which are required for enzyme activity and show cell cycle-dependent regulation. The TATA-less promoter of the human RRM1 gene (encodes R1 protein) was examined with reference to regulatory domains upstream of the transcription start site. A region from nt -195 to +3 was found to give maximal expression of a reporter gene when transfected into the human cell line K562. Overall, this 198-bp region shows 58% identity with the equivalent region of the murine promoter; however, it contains two 22-bp domains that were 81 and 91% identical between species. Electrophoretic mobility shift assays were performed using a fragment of the domain closest to the transcription start site. These experiments revealed that several factors were able to bind this region in a sequence-specific manner. One of these factors was shown to be Spl by specific competition and supershift using antibody to Spl. The data presented suggest that Spl is involved in the transcription of RRRM1. (C) 1995 Academic Press, Inc.
Publisher: ACADEMIC PRESS INC JNL-COMP SUBSCRIPTIONS
Keywords: RNA POLYMERASE-II; TRANSCRIPTION INITIATION; EXPRESSION; PROTEIN-M2; CELLS
Publisher's Version: https://doi.org/10.1006/geno.1995.1043
Terms of Use/Rights Notice: Refer to copyright notice on published article.

Creation Date: 1995-05-20 12:00:00