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小鼠X染色体上Hyp突变的精细遗传定位。

Fine genetic mapping of the Hyp mutation on mouse chromosome X.

作者信息

Du L, Desbarats M, Cornibert S, Malo D, Ecarot B

机构信息

Genetics Unit, Shriners Hospital, McGill University, Montreal, Quebec, Canada.

出版信息

Genomics. 1996 Mar 1;32(2):177-83. doi: 10.1006/geno.1996.0103.

Abstract

The hypophosphatemic (Hyp) mouse is the murine homolog of hypophosphatemic vitamin-D-resistant rickets (HYP) in human. Despite extensive investigations in the Hyp mouse, the pathophysiology of this X-linked dominant disorder remains unclear. As a first step toward cloning the Hyp gene, we have generated a high-resolution linkage map in the vicinity of the Hyp locus using two independent backcross panels segregating the Hyp mutation, one generated from an interspecific mating between C57BL/6J-Hyp/Hyp and Mus spretus and the other from an intrasubspecific mating between C57BL/6J-Hyp/Hyp and Mus musculus castaneus. Linkage analyses in 1101 backcross progeny using a total of 23 DNA markers favor the following gene order from the centromere: DXMitl3-(DXMit11, DXMit34)-(DXMit36, Alas2)-(Hyp, DXMit8O)-DXMi198-(DXMit28, DXMit33, DXMit7O)-Pdhal-DXMit2O. This study has localized Hyp to a region of approximately 1 cM flanked by the proximal markers DXMit36 and Alas2 and the distal marker DXMit98. One microsatellite marker, DXMit8O, was found to be very tightly linked to Hyp, as it was nonrecombinant with Hyp among all the progeny of both backcrosses corresponding to 1101 meioses.

摘要

低磷血症(Hyp)小鼠是人类低磷血症性维生素D抵抗性佝偻病(HYP)的小鼠同源物。尽管对Hyp小鼠进行了广泛研究,但这种X连锁显性疾病的病理生理学仍不清楚。作为克隆Hyp基因的第一步,我们利用两个独立的回交群体生成了Hyp基因座附近的高分辨率连锁图谱,一个群体是由C57BL/6J-Hyp/Hyp与小家鼠杂交产生的,另一个群体是由C57BL/6J-Hyp/Hyp与栗色小家鼠进行种内杂交产生的。使用总共23个DNA标记对1101个回交后代进行连锁分析,结果支持从着丝粒起的以下基因顺序:DXMitl3-(DXMit11,DXMit34)-(DXMit36,Alas2)-(Hyp,DXMit8O)-DXMi198-(DXMit28,DXMit33,DXMit7O)-Pdhal-DXMit2O。本研究已将Hyp基因定位到一个约1厘摩的区域,其两侧分别是近端标记DXMit36和Alas2以及远端标记DXMit98。发现一个微卫星标记DXMit8O与Hyp紧密连锁,因为在两个回交的所有后代(对应1101次减数分裂)中,它与Hyp均无重组。

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