Disclosure of five breakpoints in a complex chromosome rearrangement by microdissection and FISH

被引：5

作者：

Engelen, JJM ^{[1
]}

Loots, WJG ^{[1
]}

Albrechts, JCM ^{[1
]}

Motoh, PCC ^{[1
]}

Fryns, JP ^{[1
]}

Hamers, AJH ^{[1
]}

Geraedts, JPM ^{[1
]}

机构：

[1] KATHOLIEKE UNIV LEUVEN HOSP,CTR HUMAN GENET,LOUVAIN,BELGIUM

来源：

JOURNAL OF MEDICAL GENETICS | 1996年 / 33卷 / 07期

关键词：

chromosome microdissection; complex chromosome rearrangement (CCR); degenerate oligonucleotide primer-PCR (DOP-PCR);

D O I：

10.1136/jmg.33.7.562

中图分类号：

Q3 [遗传学];

学科分类号：

071007 ; 090102 ;

摘要：

Microdissection and fluorescence in situ hybridisation (FISH) were used to elucidate the nature of a complex chromosome translocation, after GTG banding failed in the complete characterisation of the structural rearrangement between chromosomes 6 and 12. These chromosomes were painted with chromosome specific paints and one of the chromosome regions involved in the translocation was isolated by microdissection. Ten copies of the microdissected region were collected with microneedles from GTG banded metaphases, transferred to a collecting drop, and amplified by means of DOP-PCR. The PCR product was labelled with biotin-14-dATP and used as a FISH probe for hybridisation to normal metaphase chromosomes and metaphase chromosomes of the patients (microFISH). FISH with this chromosome region specific painting probe and with chromosome band specific probes enabled the characterisation of a complex chromosome rearrangement with five breakpoints in two chromosomes. This resulted in the following karyotype: 46,XY,t(6;12) (bpter-->6q12::12q24.1-->12qter;12pter-->12q13.3::6q16.2-->6q26::12q13.3-->12q24.1::6q12-->6q16.2::6q26-->6qter).

引用

页码：562 / 566

页数：5

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