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与al相关的75千碱基缺失的物理和遗传特征,al是小鼠刺鼠基因座上的一个隐性致死等位基因。

Physical and genetic characterization of a 75-kilobase deletion associated with al, a recessive lethal allele at the mouse agouti locus.

作者信息

Barsh G S, Epstein C J

机构信息

Department of Pediatrics, University of California, San Francisco 94143.

出版信息

Genetics. 1989 Apr;121(4):811-8. doi: 10.1093/genetics/121.4.811.

Abstract

The agouti locus (A) of the mouse determines the timing and type of pigment deposition in the growing hair bulb, and several alleles at this locus are lethal when homozygous. Apparent instances of intragenic recombination and complementation between different recessive lethal alleles have suggested that the locus has a complex structure. We have begun to investigate the molecular basis of agouti gene action and recessive lethality by using a series of genetically linked DNA probes and pulsed field gel electrophoresis to detect structural alterations in radiation-induced agouti mutations. Hybridization probes from the Src and Emv-15 loci do not reveal molecular alterations in DNA corresponding to the ae, ax, and al alleles, but a probe from the parotid secretory protein gene (Psp) detects a 75-kilobase (kb) deletion in DNA containing the non-agouti lethal allele (al). The deletion is defined by a 75-kb reduction in the size of BssHII, NotI, NruI and SacII high molecular weight restriction fragments detected with the Psp probe and is located between 25 kb and 575 kb from Psp coding sequences. Because the genetic distance between A and Emv-15 is much less than A and Psp, there may be a preferred site of recombination close to Psp, or suppression of recombination between A and Emv-15. The al deletion has allowed us to determine the genotype of mice heterozygous for different recessive lethal alleles. We find that three different recessive lethal complementation groups are present at the agouti locus, two of which are contained within the al deletion.

摘要

小鼠的刺豚鼠基因座(A)决定了生长中的毛球中色素沉积的时间和类型,该基因座的几个等位基因在纯合时是致死的。不同隐性致死等位基因之间明显的基因内重组和互补实例表明该基因座具有复杂的结构。我们已开始通过使用一系列遗传连锁的DNA探针和脉冲场凝胶电泳来检测辐射诱导的刺豚鼠突变中的结构改变,从而研究刺豚鼠基因作用和隐性致死的分子基础。来自Src和Emv-15基因座的杂交探针未揭示与ae、ax和al等位基因相对应的DNA中的分子改变,但来自腮腺分泌蛋白基因(Psp)的探针检测到含有非刺豚鼠致死等位基因(al)的DNA中有一个75千碱基(kb)的缺失。该缺失由用Psp探针检测到的BssHII、NotI、NruI和SacII高分子量限制性片段大小减少75 kb来界定,并且位于距Psp编码序列25 kb至575 kb之间。由于A与Emv-15之间的遗传距离远小于A与Psp之间的距离,可能在靠近Psp处存在一个优先重组位点,或者A与Emv-15之间的重组受到抑制。al缺失使我们能够确定不同隐性致死等位基因杂合小鼠的基因型。我们发现刺豚鼠基因座存在三个不同的隐性致死互补组,其中两个包含在al缺失内。

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