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Sequence and Analysis of the Human ABL Gene, the BCR Gene, and Regions Involved in the Philadelphia Chromosomal Translocation

生物 外显子 遗传学 阿布勒 断点群集区域 粘粒 22号染色体 基因 同源(生物学) 慢性粒细胞白血病 断点 费城染色体 内含子 染色体易位 分子生物学 白血病 信号转导 酪氨酸激酶
作者
Stephanie L. Chissoe,Angelika Bodenteich,Yunfang Wang,Ying‐Ping Wang,Dennis Burian,Sandra W. Clifton,Judy S. Crabtree,Alexandra F. Freeman,Kala Iyer,Jianlin Li,Yichen Ma,Hei-Jen McLaury,Huaqin Pan,Omayma H. Sarhan,Steve Toth,Zhili Wang,Guozhong Zhang,Nora Heisterkamp,J Groffen,Bruce A. Roe
出处
期刊:Genomics [Elsevier]
卷期号:27 (1): 67-82 被引量:215
标识
DOI:10.1006/geno.1995.1008
摘要

The complete human BCR gene (152-141 nt) on chromosome 22 and greater than 80% of the human ABL gene (179-512 nt) on chromosome 9 have been sequenced from mapped cosmid and plasmid clones via a shotgun strategy. Because these two chromosomes are translocated with breakpoints within the BCR and ABL genes in Philadelphia chromosome-positive leukemias, knowledge of these sequences also might provide insight into the validity of various theories of chromosomal rearrangements. Comparison of these genes with their cDNA sequences reveal the positions of 23 BCR exons and putative alternative BCR first and second exons, as well as the common ABL exons 2-11, respectively. Additionally, these regions include the alternative ABL first exons 1b and 1a, a new gene 5' to the first ABL exon, and an open reading frame with homology to an EST within the BCR fourth intron. Further analysis reveals an Alu homology of 38.83 and 39.35% for the BCR and ABL genes, respectively, with other repeat elements present to a lesser extent. Four new Philadelphia chromosome translocation breakpoints from chronic myelogenous leukemia patients also were sequenced, and the positions of these and several other previously sequenced breakpoints now have been mapped precisely, although no consistent breakpoint features immediately were apparent. Comparative analysis of genomic sequences encompassing the murine homologues to the human ABL exons 1b and 1a, as well as regions encompassing the ABL exons 2 and 3, reveals that although there is a high degree of homology in their corresponding exons and promoter regions, these two vertebrate species show a striking lack of homology outside these regions.
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