J S Kadandale, S S Wachtel, Y Tunca, R S Wilroy, P R Martens, A T Tharapel
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引用次数: 36
摘要
引物原位标记(Primed in situ labeling, PRINS)可用于定位小到荧光原位杂交无法检测到的DNA片段。通过PRINS,我们在两名XX男性,一名患有XY性腺发育不良的女性和一名患有Xp-Yp交换的无精子男性中发现了SRY基因。由于PRINS已广泛用于重复序列的研究,我们对该技术进行了改进,以研究单拷贝2。1kb SRY序列。在XY正常男性和XY性腺发育不良女性中,在Yp11.31p11.32位点发现了SRY信号。一个XX雄性在Xp22上发现了SRY信号,而另一个在Xp22上没有。在无精子雄性的Xp-Yp交换的der(X)的相应区域(Xp22)中鉴定出它们。正常XX女性未见SRY信号。聚合酶链反应证实了不同受试者DNA样本中SRY的存在。总的来说,PRINS是快速定位单拷贝基因和小DNA片段的理想选择。
Localization of SRY by primed in situ labeling in XX and XY sex reversal.
Primed in situ labeling (PRINS) can be used to localize DNA segments too small to be detected by fluorescence in situ hybridization. By PRINS we identified the SRY gene in two XX males, a woman with XY gonadal dysgenesis, and an azoospermic male with Xp-Yp interchange. Because PRINS has been used generally in the study of repetitive sequences, we modified the technique for study of the single copy 2. 1-kb SRY sequence. SRY signals were identified at band Yp11.31p11.32 in normal XY males and in the woman with XY gonadal dysgenesis. SRY signals were identified on Xp22 in one XX male but not in the other. They were identified in the corresponding region (Xp22) of the der(X) in the azoospermic male with Xp-Yp interchange. SRY signals were not observed in normal XX females. Presence of SRY in DNA samples from the various subjects was confirmed by polymerase chain reaction. We conclude that PRINS is ideal for rapid localization of single copy genes and small DNA segments in general.
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