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小鼠髓鞘碱性蛋白基因突变(颤抖者)和正常等位基因的植入前快速检测,可实现选择性植入并产下存活幼崽。

Rapid preimplantation detection of mutant (shiverer) and normal alleles of the mouse myelin basic protein gene allowing selective implantation and birth of live young.

作者信息

Gomez C M, Muggleton-Harris A L, Whittingham D G, Hood L E, Readhead C

机构信息

Division of Biology, California Institute of Technology, Pasadena 91125.

出版信息

Proc Natl Acad Sci U S A. 1990 Jun;87(12):4481-4. doi: 10.1073/pnas.87.12.4481.

Abstract

As a model for the detection of human genetic disease in preimplantation embryos, we describe a method in which trophectoderm biopsy samples from viable mouse blastocysts are simultaneously analyzed for the presence of a normal or mutant allele of the myelin basic protein gene by the polymerase chain reaction. The biopsied embryos are kept in culture during analysis of biopsied material and later reintroduced to a foster mother. Prenatal diagnosis can be completed in less than 7 hr. The identity of either amplification product was proved conclusively by direct sequence analysis of amplified products. Ninety-six percent of recovered blastocysts survived biopsy, as judged by re-formation of a blastocyst cavity in culture. Fifty-nine percent of the biopsied embryos established pregnancy by day 6.5, compared to 88% of unmanipulated controls. This approach can be applied to preimplantation diagnosis of human genetic diseases by using extraembryonic cells from blastocysts obtained after in vitro fertilization or uterine lavage. It will make possible the elimination of a mutant allele from a family in a single generation.

摘要

作为检测植入前胚胎中人类遗传疾病的模型,我们描述了一种方法,即通过聚合酶链反应同时分析来自存活小鼠囊胚的滋养外胚层活检样本中髓鞘碱性蛋白基因正常或突变等位基因的存在情况。在对活检材料进行分析期间,将活检后的胚胎保存在培养液中,随后再植入代孕母体。产前诊断可在不到7小时内完成。通过对扩增产物进行直接序列分析,最终确定了两种扩增产物的身份。根据培养中囊胚腔的重新形成判断,96%的回收囊胚在活检后存活。到第6.5天时,59%的活检胚胎成功着床,而未进行操作的对照胚胎着床率为88%。该方法可应用于人类遗传疾病的植入前诊断,通过使用体外受精或子宫灌洗后获得的囊胚中的胚外细胞。这将有可能在一代人的时间内从一个家族中消除突变等位基因。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/7d76/54139/83b9cc1b3f0d/pnas01037-0079-a.jpg

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