The basic helix-loop-helix protein upstream stimulating factor regulates the cardiac ventricular myosin light-chain 2 gene via independent cis regulatory elements.

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Mol Cell Biol. 1994 November; 14(11): 7331-7339

The basic helix-loop-helix protein upstream stimulating factor regulates the cardiac ventricular myosin light-chain 2 gene via independent cis regulatory elements.

S Navankasattusas, M Sawadogo, M van Bilsen, C V Dang and K R Chien

Biomedical Science Program, University of California-San Diego, La Jolla 92093.

ABSTRACT

Previous studies have documented that 250 bp of the rat cardiacventricular myosin light-chain 2 (MLC-2v) promoter is sufficientto confer cardiac muscle-specific expression on a luciferasereporter gene in both transgenic mice and primary cultured neonatalrat myocardial cells. Utilizing ligation-mediated PCR to performin vivo dimethyl sulfate footprinting, the present study hasidentified protein-DNA interaction within the position from-176 to -165. This region, identified as MLE1, contains a coresequence, CACGTG, which conforms to the consensus E-box siteand is identical to the upstream stimulating factor (USF)-bindingsite of the adenovirus major late promoter. Transient assaysof luciferase reporter genes containing point mutations of thesite demonstrate the importance of this cis regulatory elementin the transcriptional activation of this cardiac muscle genein ventricular muscle cells. The protein complex that occupiesthis site is capable of binding to HF-1a and PRE B sites whichare known to be required for cardiac muscle-specific expressionof rat MLC-2v and alpha-myosin heavy-chain genes, respectively.This study provides direct evidence that USF, a member of thebasic helix-loop-helix leucine zipper family, binds to MLE1,HF-1a, and PRE B sites and suggests that it is a component ofprotein complexes that may coordinately control the expressionof MLC-2v and alpha-myosin heavy-chain genes. The current studyalso provides evidence that USF can positively and negativelyregulate the MLC-2v gene via independent cis regulatory elements.

Mol Cell Biol. 1994 November; 14(11): 7331-7339

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