首页> 美国卫生研究院文献>Springer Open Choice >Cryopreservation enhances embryogenic capacity of Gentiana cruciata (L.) suspension culture and maintains (epi)genetic uniformity of regenerants
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Cryopreservation enhances embryogenic capacity of Gentiana cruciata (L.) suspension culture and maintains (epi)genetic uniformity of regenerants

机译:冷冻保存增强了Gentiana cruciata(L.)悬浮培养的胚发生能力并保持了再生剂的(epi)遗传均一性

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摘要

The embryogenic cell suspension culture of Gentiana cruciata, cryopreserved by the encapsulation/dehydration method, survived both short- (48 h) and long-term (1.5 years) cryostorage with more than 80% viability. To assess the influence of cryotreatments on the embryogenic potential, a proembryogenic mass was encapsulated and exposed to the following treatments: (1) osmotic dehydration (OD), (2) OD + air desiccation (AD) and (3) OD + AD + cryostorage (LN). The somatic embryogenesis efficiency increased ten times after osmotic dehydration. The AD and LN cryotreatments did not cause any significant alterations in somatic embryo production. We monitored the (epi)genetic stability of 288 regenerants derived from: non-cryotreated, short-term, and long-term cryostored tissue using metAFLP markers and ten primer combinations. Changes in the sequence and DNA methylation levels were studied by subjecting the DNA to digestion with two pairs of isoschisomer restriction enzymes (KpnI/MseI and Acc65I/MseI). Two new AFLP unique DNA fragments at the DNA sequence level, with no differences at the methylation level, were found between regenerants derived from cryopreserved tissue, compared with the non-cryotreated controls. The Acc65I/MseI methylation levels for the three groups of regenerants were not significantly different. Cluster analysis was capable of identifying a number of sub-clusters. Only one of the sub-clusters comprises almost all regenerants derived from non-cryotreated and short-term cryostored tissue. Plantlets derived from long-term cryostored tissue were grouped into separate clusters. The observed AFLP alterations did not appear to be associated with the use of cryopreservation, but were probably related to the process of in vitro culture.
机译:通过包囊/脱水方法冷冻保存的Gentiana cruciata的胚胎发生细胞悬浮培养物在短期(48小时)和长期(1.5年)冷冻保存中均存活,存活率超过80%。为了评估冷冻处理对胚胎发生潜能的影响,将促胚团包裹并进行以下处理:(1)渗透脱水(OD),(2)OD +空气干燥(AD)和(3)OD + AD +冷冻箱(LN)。渗透脱水后,体细胞胚胎发生效率提高了十倍。 AD和LN冷冻处理并未引起体细胞胚胎产生任何重大变化。我们使用metAFLP标记和十种引物组合监测了288种再生子的(epi)遗传稳定性,这些再生子来自:未低温处理,短期和长期冷冻保存的组织。通过用两对同分异构酶限制酶(KpnI / MseI和Acc65I / MseI)消化DNA来研究序列和DNA甲基化水平的变化。与未冷冻处理的对照相比,在低温保存的组织衍生的再生体之间发现了两个新的AFLP独特的DNA片段,其DNA序列水平在甲基化水平上没有差异。三组再生剂的Acc65I / MseI甲基化水平没有显着差异。聚类分析能够确定许多子类。子簇中只有一个包含几乎所有衍生自未经冷冻和短期冷冻保存的组织的再生剂。来自长期低温保存组织的小植株被分为单独的簇。观察到的AFLP改变似乎与冷冻保存的使用无关,但可能与体外培养的过程有关。

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