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5S核糖体DNA的物理图谱揭示了3R染色体上的一个新位点以及用于染色体作图的黑麦易位系中意想不到的复杂性。

Physical mapping of 5S rDNA reveals a new locus on 3R and unexpected complexity in a rye translocation used in chromosome mapping.

作者信息

Alonso-Blanco C, Pendás A M, Garcia-Suarez R, Roca A, Goicoechea P G, Giraldez R

机构信息

Departamento de Biología Funcional, Universidad de Oviedo, Spain.

出版信息

Chromosoma. 1994 Sep;103(5):331-7. doi: 10.1007/BF00417880.

DOI:10.1007/BF00417880
PMID:7821088
Abstract

Using fluorescence in situ hybridization (FISH) with probe pScT7, three different 5S rDNA loci were detected in the satellite of rye chromosome 1R (5SDna-R1) and in the short arms of chromosomes 3R (5SDna-R3) and 5R (5SDna-R2) respectively. All three loci showed polymorphism for the hybridization signal intensity. In order to determine the localization of these rye 5S rDNA multigene loci with higher precision within the corresponding chromosome arms, the probe pScT7 was physically mapped by FISH in relation to the following five translocations (Wageningen Tester Set): T850W (1RS/4RL), T248W (1RS/6RS), T273W (1RS/5RL), T305W (2RS/5RS) and T240W (3RS/5RL). Accurate physical maps of the translocation breakpoints had previously been made using electron microscope analysis of spread pachytene synaptonemal complexes of heterozygotes for the different translocations. The results indicate that locus 5SDna-R3 is located between the breakpoint of translocation T240W and the telomere, whereas locus 5SDna-R2 is located between the breakpoint of translocation T305W and the centromere, the hybridization of probe pScT7 on T305W translocated chromosomes demonstrating the complex nature of this translocation. On the other hand, the simultaneous detection of probes pScT7 and pTA71 (18S-5.8S-26S rDNA) with two different fluorochromes, indicated that the breakpoints of translocations T850W and T248W are located between loci Nor-R1 and 5SDna-R1.

摘要

使用探针pScT7进行荧光原位杂交(FISH),在黑麦1R染色体的随体(5SDna - R1)以及3R染色体(5SDna - R3)和5R染色体(5SDna - R2)的短臂上分别检测到三个不同的5S rDNA位点。所有这三个位点的杂交信号强度均表现出多态性。为了更精确地确定这些黑麦5S rDNA多基因位点在相应染色体臂内的定位,通过FISH将探针pScT7相对于以下五个易位(瓦赫宁根测试集)进行了物理定位:T850W(1RS/4RL)、T248W(1RS/6RS)、T273W(1RS/5RL)、T305W(2RS/5RS)和T240W(3RS/5RL)。此前已通过对不同易位杂合子的伸展粗线期联会复合体进行电子显微镜分析,制作出了易位断点的精确物理图谱。结果表明,位点5SDna - R3位于易位T240W的断点与端粒之间,而位点5SDna - R2位于易位T305W的断点与着丝粒之间,探针pScT7在T305W易位染色体上的杂交显示了该易位的复杂性。另一方面,用两种不同荧光染料同时检测探针pScT7和pTA71(18S - 5.8S - 26S rDNA)表明,易位T850W和T248W的断点位于Nor - R1位点和5SDna - R1位点之间。

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本文引用的文献

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Identification of rye chromosomes: the Giemsa banding pattern and the translocation tester set.黑麦染色体的鉴定:吉姆萨带型和易位测试体系。
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Mapping seed storage protein loci Sec-1 and Sec-3 in relation to five chromosomal rearrangements in rye (Secale cereale L.).定位与黑麦五个染色体重排有关的种子贮藏蛋白基因座 Sec-1 和 Sec-3。
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A cytogenetic map on the entire length of rye chromosome 1R, including one translocation breakpoint, three isozyme loci and four C-bands.一个包含一个易位断点、三个同工酶位点和四个 C 带的整条黑麦 1R 染色体的细胞遗传学图谱。
Theor Appl Genet. 1993 Feb;85(6-7):735-44. doi: 10.1007/BF00225013.
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Physical mapping of translocation breakpoints in rye by means of synaptonemal complex analysis.利用联会复合体分析对黑麦易位断点进行物理作图。
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A cytogenetically based physical map of chromosome 1B in common wheat.普通小麦 1B 染色体基于细胞遗传学的物理图谱。
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9
Physical mapping of four sites of 5S rDNA sequences and one site of the α-amylase-2 gene in barley (Hordeum vulgare).大麦(Hordeum vulgare)中 5S rDNA 序列的四个位点和α-淀粉酶-2 基因的一个位点的物理作图。
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