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Identification and characterization of functional genes encoding the mouse major urinary proteins.

机译:鉴定和表征编码小鼠主要尿蛋白的功能基因。

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摘要

Mouse Ltk- cells were stably transfected with cloned genes encoding the mouse major urinary proteins (MUPs). C57BL/6J MUP genomic clones encoding MUP 2 (BL6-25 and BL6-51), MUP 3 (BL6-11 and BL6-3), and MUP 4 (BL6-42) have been identified. In C57BL/6J mice, MUP 2 and MUP 4 are known to be synthesized in male, but not female, liver, and MUP 3 is known to be synthesized in both male and female liver and mammary gland. A BALB/c genomic clone (BJ-31) was shown to encode a MUP that is slightly more basic than MUP 2 and was previously shown to be synthesized in both male and female liver of BALB/c but not C57BL/6 mice. Comigration on two-dimensional polyacrylamide gels of the MUPs encoded by the transfecting gene provides a basis for tentative identification of the tissue specificity and mode of regulation of each gene. DNA sequence analysis of the 5' flanking region indicates that the different MUP genes are highly homologous (0.20 to 2.40% divergence) within the 879 base pairs analyzed. The most prominent differences in sequence occur within an A-rich region just 5' of the TATA box. This region (from -47 to -93) contains primarily A or C(A)N nucleotides and varies from 15 to 46 nucleotides in length in the different clones.
机译:小鼠Ltk细胞被编码小鼠主要尿蛋白(MUPs)的克隆基因稳定转染。已鉴定出编码MUP 2(BL6-25和BL6-51),MUP 3(BL6-11和BL6-3)和MUP 4(BL6-42)的C57BL / 6J MUP基因组克隆。在C57BL / 6J小鼠中,已知MUP 2和MUP 4在雄性肝脏中合成,但不是在雌性肝脏中合成,并且MUP 3在雄性,雌性肝脏和乳腺中合成。已显示BALB / c基因组克隆(BJ-31)编码的MUP比MUP 2基本碱性,并且先前已显示可在BALB / c的雄性和雌性肝脏中合成,但未在C57BL / 6小鼠中合成。在转染基因编码的MUP的二维聚丙烯酰胺凝胶上的交换为初步鉴定每个基因的组织特异性和调控模式提供了基础。 5'侧翼区的DNA序列分析表明,在所分析的879个碱基对中,不同的MUP基因具有高度同源性(0.20至2.40%的差异)。序列上最显着的差异发生在TATA盒5'端的A富集区域内。该区域(从-47到-93)主要包含A或C(A)N核苷酸,并且在不同克隆中的长度在15到46个核苷酸之间。

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