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用荧光原位杂交技术对蓝花葱愈伤组织再生植株进行染色体分析

Chromosome analysis by fluorescence in situ hybridization of callus-derived regenerants in Allium cyaneum R.

作者信息

Lee S H, Ryu J A, Do G S, Seo B B, Pak J H, Kim I S, Song S D

机构信息

Department of Biology, Kyungpook National University, Taegu 702-701, Korea Fax: +82-53-953-3066 e-mail:

Department of Biology, Keimyung University, Taegu 704-701, Korea, , , , , , KR.

出版信息

Plant Cell Rep. 1998 Dec;18(3-4):209-213. doi: 10.1007/s002990050558.

DOI:10.1007/s002990050558
PMID:30744222
Abstract

Investigations were performed to confirm the optimal in vitro culture condition for callus induction and plant regeneration, to observe if somoclonal variation occurs among regenerated plants at the ploidy level and to analyse the chromosomal location of 5S and 18S-26S rRNA gene families using fluorescence in situ hybridization in callus-derived plants of Allium cyaneum. High-est callus initiation was achieved with bulb explants cultured on MS medium supplemented with 2,4-D and BAP at 1 mg l each. A total of 195 plants was obtained when using MS medium supplemented with 1 mg l NAA and 5 mg l BAP; about 92% were diploid having 2n=16; 8% showed a variation in ploidy level. Using digoxigenin-labelled 5S rRNA and biotin-labelled 18S-26S rRNA gene probes, we compared the fluorescence in situ hybridization patterns of autotetraploid plants with the A. cyaneum wild type. The 5S rRNA gene sites were detected on the interstitial region in the short arm of chromosome 4 and on the interstitial region in both arms of chromosome 7. The 18S-26S rRNA gene sites were detected on the terminal region of the short arm, including the satellite of chromosome 5, as well as on a part of chromosome B. The chromosomal location of both rRNA genes in regenerated autotetraploid plants corresponded to those of the wild species.

摘要

进行了多项研究,以确定用于愈伤组织诱导和植株再生的最佳体外培养条件,观察再生植株在倍性水平上是否发生体细胞克隆变异,并利用荧光原位杂交技术分析蓝花葱愈伤组织衍生植株中5S和18S - 26S rRNA基因家族的染色体定位。在添加了1 mg/L 2,4 - D和1 mg/L BAP的MS培养基上培养鳞茎外植体时,愈伤组织诱导率最高。使用添加了1 mg/L NAA和5 mg/L BAP的MS培养基时,共获得了195株植株;约92%为二倍体,2n = 16;8%表现出倍性水平的变异。使用地高辛标记的5S rRNA和生物素标记的18S - 26S rRNA基因探针,我们比较了同源四倍体植株与蓝花葱野生型的荧光原位杂交模式。在染色体4短臂的中间区域和染色体7双臂的中间区域检测到了5S rRNA基因位点。在染色体5短臂的末端区域,包括卫星区域,以及染色体B的一部分上检测到了18S - 2is rRNA基因位点。再生同源四倍体植株中两个rRNA基因的染色体定位与野生种的一致。

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