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从冷驯化到去驯化过程中,蓝莓叶片、发育中的果实和花芽的转录组序列的生成和分析。

Generation and analysis of blueberry transcriptome sequences from leaves, developing fruit, and flower buds from cold acclimation through deacclimation.

机构信息

Genetic Improvement of Fruits and Vegetables Laboratory, USDA-ARS, BARC-West, 10300 Baltimore Ave., Beltsville, MD 20705, USA.

出版信息

BMC Plant Biol. 2012 Apr 2;12:46. doi: 10.1186/1471-2229-12-46.

DOI:10.1186/1471-2229-12-46
PMID:22471859
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3378433/
Abstract

BACKGROUND

There has been increased consumption of blueberries in recent years fueled in part because of their many recognized health benefits. Blueberry fruit is very high in anthocyanins, which have been linked to improved night vision, prevention of macular degeneration, anti-cancer activity, and reduced risk of heart disease. Very few genomic resources have been available for blueberry, however. Further development of genomic resources like expressed sequence tags (ESTs), molecular markers, and genetic linkage maps could lead to more rapid genetic improvement. Marker-assisted selection could be used to combine traits for climatic adaptation with fruit and nutritional quality traits.

RESULTS

Efforts to sequence the transcriptome of the commercial highbush blueberry (Vaccinium corymbosum) cultivar Bluecrop and use the sequences to identify genes associated with cold acclimation and fruit development and develop SSR markers for mapping studies are presented here. Transcriptome sequences were generated from blueberry fruit at different stages of development, flower buds at different stages of cold acclimation, and leaves by next-generation Roche 454 sequencing. Over 600,000 reads were assembled into approximately 15,000 contigs and 124,000 singletons. The assembled sequences were annotated and functionally mapped to Gene Ontology (GO) terms. Frequency of the most abundant sequences in each of the libraries was compared across all libraries to identify genes that are potentially differentially expressed during cold acclimation and fruit development. Real-time PCR was performed to confirm their differential expression patterns. Overall, 14 out of 17 of the genes examined had differential expression patterns similar to what was predicted from their reads alone. The assembled sequences were also mined for SSRs. From these sequences, 15,886 blueberry EST-SSR loci were identified. Primers were designed from 7,705 of the SSR-containing sequences with adequate flanking sequence. One hundred primer pairs were tested for amplification and polymorphism among parents of two blueberry populations currently being used for genetic linkage map construction. The tetraploid mapping population was based on a cross between the highbush cultivars Draper and Jewel (V. darrowii is also in the background of 'Jewel'). The diploid mapping population was based on a cross between an F1 hybrid of V. darrowii and diploid V. corymbosum and another diploid V. corymbosum. The overall amplification rate of the SSR primers was 68% and the polymorphism rate was 43%.

CONCLUSIONS

These results indicate that this large collection of 454 ESTs will be a valuable resource for identifying genes that are potentially differentially expressed and play important roles in flower bud development, cold acclimation, chilling unit accumulation, and fruit development in blueberry and related species. In addition, the ESTs have already proved useful for the development of SSR and EST-PCR markers, and are currently being used for construction of genetic linkage maps in blueberry.

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/271a/3378433/6237175586c3/1471-2229-12-46-7.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/271a/3378433/89dd939bb258/1471-2229-12-46-1.jpg
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https://cdn.ncbi.nlm.nih.gov/pmc/blobs/271a/3378433/e623e4a25c3a/1471-2229-12-46-5.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/271a/3378433/a486f2e87520/1471-2229-12-46-6.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/271a/3378433/6237175586c3/1471-2229-12-46-7.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/271a/3378433/89dd939bb258/1471-2229-12-46-1.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/271a/3378433/e369d70af70a/1471-2229-12-46-2.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/271a/3378433/9c8f1dc29ffe/1471-2229-12-46-3.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/271a/3378433/4fdd09c67de6/1471-2229-12-46-4.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/271a/3378433/e623e4a25c3a/1471-2229-12-46-5.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/271a/3378433/a486f2e87520/1471-2229-12-46-6.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/271a/3378433/6237175586c3/1471-2229-12-46-7.jpg
摘要

背景

近年来,蓝莓的消费有所增加,部分原因是其具有许多公认的健康益处。蓝莓果实富含花青素,已被证明能改善夜视能力、预防黄斑变性、抗癌活性和降低心脏病风险。然而,蓝莓的基因组资源非常有限。进一步开发基因组资源,如表达序列标签(ESTs)、分子标记和遗传连锁图谱,可以促进遗传改良的快速发展。标记辅助选择可用于将适应气候的性状与果实和营养品质性状相结合。

结果

本文介绍了对商业高丛蓝莓(Vaccinium corymbosum)品种 Bluecrop 的转录组进行测序的努力,并利用这些序列鉴定与冷驯化和果实发育相关的基因,并开发 SSR 标记用于图谱研究。通过下一代罗氏 454 测序,从不同发育阶段的蓝莓果实、不同冷驯化阶段的花芽和叶片中生成转录组序列。将超过 600,000 个读数组装成大约 15,000 个重叠群和 124,000 个单倍体。组装的序列被注释并功能映射到基因本体论(GO)术语。比较所有文库中每个文库中最丰富序列的频率,以鉴定在冷驯化和果实发育过程中可能差异表达的基因。通过实时 PCR 验证它们的差异表达模式。总体而言,在所检查的 17 个基因中,有 14 个基因的表达模式与仅根据其读数预测的模式相似。还从这些序列中挖掘了 SSR。从这些序列中,鉴定出 15,886 个蓝莓 EST-SSR 基因座。从含有足够侧翼序列的 7,705 个 SSR 序列中设计了引物。测试了 100 对引物在用于遗传连锁图谱构建的两个蓝莓群体亲本中的扩增和多态性。四倍体图谱群体基于高丛品种 Draper 和 Jewel 的杂交('Jewel'的背景中也有 V. darrowii)。二倍体图谱群体基于 V. darrowii 和二倍体 V. corymbosum 的 F1 杂种与另一个二倍体 V. corymbosum 的杂交。SSR 引物的总体扩增率为 68%,多态性率为 43%。

结论

这些结果表明,这一大批 454 EST 将成为鉴定可能差异表达并在蓝莓及相关物种的花芽发育、冷驯化、冷量积累和果实发育中发挥重要作用的基因的宝贵资源。此外,EST 已经证明对 SSR 和 EST-PCR 标记的开发有用,并且目前正在用于蓝莓的遗传连锁图谱构建。

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