Myosin II protein molecules, which consist of a pair of heavy chains (approximately 200 kDa) and two pairs of light chains (15-28 kDa), exist in all eukaryotic cells. Together with actin filaments, they produce contractile force mediated by ATP hydrolysis. While this contractile activity is prominent in differentiated muscle tissues, it is also involved in diverse cellular motile processes such as cytokinesis, cell migration and cell adhesion in nonmuscle cells, as well as in undifferentiated muscle cells. In vertebrates, there are over 10 different myosin II isoforms, each of which contains different myosin II heavy chains (MHCs). MHC isoform diversity is generated by multiple genes as well as by alternative splicing of pre-mRNA. Previous studies have demonstrated cell type-specific expression of MHC isoforms as well as changes in MHC isoforms during the course of muscle and nervous tissue development. This research program has investigated the regulatory mechanisms responsible for the expression of two nonmuscle MHC genes, NMHC-A and NMHC-B. We have focused on NMHC-A gene regulation as it relates to cell type-dependent transcriptional mechanisms and NMHC-B gene regulation as it relates to neural cell-specific alternative pre-mRNA splicing mechanisms. With respect to NMHC-A gene regulation, the region extending 20 kb upstream and 40 kb downstream (which includes the 39 kb intron 1) from the transcriptional start sites were examined by reporter gene analysis, in an attempt to identify cis-regulatory elements. A number of regions located in intron 1 were found to modulate transcription in a cell type-dependent manner. In this study, we focused on a 0.5 kb fragment located 33 kb downstream from the transcriptional start sites. Sequence comparisons between the human and mouse genes revealed high levels of conservation in a region of 150 bp within the 0.5 kb fragment. Further reporter gene analysis and electrophoretic mobility shift assays defined an ISRE element as a major regulatory element. Among a large family of IRF proteins, IRF-2 was found to bind this element in vitro and in intact cells. With respect to NMHC-B, previous studies in this laboratory have demonstrated the existence of a neural cell-specific NMHC-B isoform, in addition to the ubiquitously expressed form of NMHC-B. This neural cell-specific isoform is generated by alternative splicing of a single cassette type of exon N30 which is located between constitutive exons E5 and E6. To characterize regulatory elements required for alternative splicing of N30, neural retinoblastoma Y79 cells, which are capable of including N30 to a large extent during postmitotic and differentiated states, were used as a model system. A cis-acting intronic enhancer (IDDE), located approximately 1.5 kb downstream of N30, and an exonic enhancer located within N30, were found to be indispensable for neural cell-specific inclusion of N30. The IDDE activates the upstream E5-N30 splicing in vitro by facilitating early prespliceosome complex formation. In contrast, the IDDE has no effect on the downstream N30-E6 splicing where the IDDE resides. An RNA-binding protein, ataxin 2-binding protein (A2BP1), has been reported to be expressed exclusively in brain, heart, and skeletal muscle and to interact with ataxin 2, which is a product of the causative gene for spinocerebellar ataxin type 2. Cotransfection of the A2BP1 expression construct with minigene reporter constructs showed that A2BP1 was capable of activating N30 inclusion in an IDDE-dependent manner.

Agency
National Institute of Health (NIH)
Institute
National Heart, Lung, and Blood Institute (NHLBI)
Type
Intramural Research (Z01)
Project #
1Z01HL004225-10
Application #
6690558
Study Section
(LMC)
Project Start
Project End
Budget Start
Budget End
Support Year
10
Fiscal Year
2002
Total Cost
Indirect Cost
Name
U.S. National Heart Lung and Blood Inst
Department
Type
DUNS #
City
State
Country
United States
Zip Code