Construction and characterization of normalized cDNA library of maize inbred MO17 from multiple tissues and developmental stages

Zhang, Z. X.; Zhang, F. D.; Tang, Wanhu; Pi, Yan; Zheng, Younglian

doi:10.1007/s11008-005-0026-8

Cited by 4 publications

(3 citation statements)

References 26 publications

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“…Although, there are several strategies that could be utilized for normalization (Ko 1990;Soares et al 1994), a new method based on saturation hybridization with genomic DNA has been effectively used in rice and maize (Chu et al 2003;Zhang et al 2005). In our study, this approach was followed to construct a normalized cDNA library of TPGMS wheat.…”

Section: Discussionmentioning

confidence: 99%

Construction, Characterization, and Expressed Sequence Tag (EST) Analysis of Normalized cDNA Library of Thermo-Photoperiod-Sensitive Genic Male Sterile (TPGMS) Wheat from Spike Developmental Stages

et al. 2008

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Thermo-photoperiod-sensitive genic male sterile (TPGMS) wheat is important in utilization of heterosis. To facilitate the use of such wheat line in agriculture, more knowledge about molecular mechanisms of TPGMS genes is required. In this study, we set up a normalized complementary DNA (cDNA) library based on the strategy of saturation hybridization with genomic DNA using TPGMS wheat line. This normalized cDNA library consists of cDNA from six directionally cloned cDNA libraries constructed with spike and anther tissues from spike developmental stages. From the normalized cDNA library, 3,264 single-pass expressed sequence tag (EST) were obtained. Exclusion of sequences shorter than 100 bp resulted in 3,223 vector-trimmed ESTs with a mean length of 926 bp. Clustering and assembly analysis resulted in 2,175 unique ESTs from 423 contigs and 1,752 singletons. Taking advantage of various tools and database, gene function classification showed that 60% of the ESTs were predicted to have putative gene function. Of the 2,175 unique ESTs, 264 (12%) displayed significant homology (BlastX E values <10 −5 ) to genes previously reported to be involved in cold-response related processes. Among these, sequences encoding activities related to primary metabolism, signal transduction, and transcriptional regulation were observed. Finally, in the total EST sequences, 108 potential SSRs were found. The unigene dataset will now be used to fabricate biochips carrying all identified genes for TPGMS wheat functional genomic research.

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Section: Discussionmentioning

confidence: 99%

Construction, Characterization, and Expressed Sequence Tag (EST) Analysis of Normalized cDNA Library of Thermo-Photoperiod-Sensitive Genic Male Sterile (TPGMS) Wheat from Spike Developmental Stages

et al. 2008

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“…Reverse transcription primers were a combination of 5SM4Z, 5SM4ZA, and 5SM4ZB in a ratio of 1:1:1 (5SM4Z: GCC ATT ACG GCC AAG TTA C XXXX X-3′, 5SM4ZA: GCC ATT ACG GCC AAG TTA C XXXX-3′, 5SM4ZB: GCC ATT ACG GCC AAG TTA C XXX-3′, X = modified G). Subsequently, normalization was performed according to Patanjali et al (1991) , Soares et al (1994) , Zhang et al (2005) , and Li et al (2012) . Later, the normalized cDNAs were integrated into the pJL12 vector using T4 DNA ligase (Thermo Scientific) and transformed into DH5α for propagation and storage.…”

Section: Methodsmentioning

confidence: 99%

Large-Scale Investigation of Soybean Gene Functions by Overexpressing a Full-Length Soybean cDNA Library in Arabidopsis

Huang

Lü

et al. 2018

Front. Plant Sci.

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Molecular breeding has become an important approach for crop improvement, and a prerequisite for molecular breeding is elucidation of the functions of genetic loci or genes. Soybean is one of the most important food and oil crops worldwide. However, due to the difficulty of genetic transformation in soybean, studies of its functional genomics lag far behind those of other crops such as rice, which severely impairs the progress of molecular improvement in soybean. Here, we describe an effective large-scale strategy to investigate the functions of soybean genes via overexpression of a full-length soybean cDNA library in Arabidopsis. The overexpression vector pJL12 was modified for use in the construction of a normalized full-length cDNA library. The constructed cDNA library showed good quality; repetitive clones represented approximately 4%, insertion fragments were approximately 2.2 kb, and the full-length rate was approximately 98%. This cDNA library was then overexpressed in Arabidopsis, and approximately 2000 transgenic lines were preliminarily obtained. Phenotypic analyses of the positive T1 transgenic plants showed that more than 5% of the T1 transgenic lines displayed abnormal developmental phenotypes, and approximately 1% of the transgenic lines exhibited potentially favorable traits. We randomly amplified 4 genes with obvious phenotypes (enlarged seeds, yellowish leaves, more branches, and dense siliques) and repeated the transgenic analyses in Arabidopsis. Subsequent phenotypic observation demonstrated that these phenotypes were indeed due to the overexpression of soybean genes. We believe our strategy represents an effective large-scale approach to investigate the functions of soybean genes and further reveal genes favorable for molecular improvement in soybean.

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“…原料。由于我国人多地少, 粮棉争地的矛盾非常突出。短季棉品种由于生育期短、开花结铃集中、简化管理的优点, 在麦棉两熟或多熟制栽培体系中发挥着重要作用 [1] 。在植物的生活周期中, 最明显的变化是营养生长到生殖生长的转变, 转折点是花芽分化。从花芽分化开始, 除一般的生理生化代谢外, 核酸代谢至关重要, 即 RNA 和 DNA 含量的积累是花器官发育的必要条件, 这已在苍耳 [2] 、牵牛 [3] 、苹果 [4] 、葡萄 [5] 等植物中得到证实。李丽等 [6] 认为, 在花芽诱导过程中, 不仅需要有较多的 RNA 和较少的 DNA, 而且还需要较高的 RNA/DNA。近年来, 已从几种模式植物, 如拟南芥 [7][8] 、金鱼草 [9] 、烟草 [10] 等分离克隆了大量与植物开花有关的调控基因。并建立起在花器官发育中同源异型基因作用的 ABC 模型 [11][12] 。全长 cDNA 是功能基因组学和比较基因组学研究的基础 [13] , 而用适当的方法筛选全长 cDNA 文库, 己成为从真核生物细胞中高效获得全长 cDNA 的有效途径。目前, 棉花在分子生物学水平上的研究还远远滞后于水稻、玉米等作物, 因此要克隆棉花中一些重要基因, 最好的途径是构建代表特定时期全部细胞表达信息的 cDNA 文库, 并从中筛选相关基因的阳性克隆。Pear 等 [14] 构建了陆地棉纤维(Acala SJ-2)的 cDNA 文库, 对棉花的 celA 基因进行了研究。Li 等 [15] 构建了陆地棉 Coker312 纤维的 cDNA 文库, 并从中得到全长 GhTUB1 cDNA。近年来, 已构建的棉花 cDNA 文库也多与棉花纤维发育时期有关 [16][17] , 用于筛选与棉花纤维品质相关基因, Ji 等 [18] 利用 subtractive PCR 和 cDNA array 分离并且分析了陆地棉徐州 142 纤维发育早期表达的基因。而棉花其他组织器官的 cDNA 文库构建相对较少。 Clontech(美国)公司推出的 SMART 技术 [19] 是目前应用最广泛的构建全长文库的方法之一。而高丰度的基因给 cDNA 文库的筛选造成了大量的重复性工作和资源浪费, 尤其不适应 EST(序列表达标签) 测序。为了解决这个问题, 开发了 cDNA 文库的均一化技术, 它降低了高丰度基因的拷贝数, 使不同丰度的基因的拷贝数趋于一致 [20] , 大大有利于目的基因的筛选和高通量的 EST 测序。DSN (duplex-specific enzyme)是近年来发现的一种热稳定核酸酶 [21]…”

Section: 棉花是我国重要的经济作物和纺织工业的重要unclassified

Establishment and Identification of a Normalized Full-Length cDNA Library of CCRI 36

Wang¹,

Liu²,

Yu³

et al. 2009

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Short season cotton (SSC) breeding plays an important role in solving the competition for more growing area between cotton and food crops. To explore the premature mechanism of SSC, to clone genes that have a close relation with premature flowering, and to speed process of premature cultivar breeding, we established a normalized full-length cDNA library using the flower and bud of CCRI 36 by DSN (duplex-specific nuclease)-normalization method combined with SMART (switching mechanism at 5' end of RNA transcript) technique. The titer of un-amplified cDNA library was about 1.7×10 6 cfu mL −1 . The average size of cDNA inserts was 1 200 bp with a recombination rate of 100%. The abundance of transcripts Histon3 and UBQ7 decreased obviously in normalized cDNA library comparing with that in non-normalized samples detected by Virtual Northern Blot. Meanwhile, protein genes associated with flower development were obtained on the basis of the positive signal of cDNA library by PCR. These results indicated that the normalized full-length cDNA library has been established successfully, which is convenient for further study on the molecular mechanism and gene cloning of flower development.

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Construction and characterization of normalized cDNA library of maize inbred MO17 from multiple tissues and developmental stages

Cited by 4 publications

References 26 publications

Construction, Characterization, and Expressed Sequence Tag (EST) Analysis of Normalized cDNA Library of Thermo-Photoperiod-Sensitive Genic Male Sterile (TPGMS) Wheat from Spike Developmental Stages

Construction, Characterization, and Expressed Sequence Tag (EST) Analysis of Normalized cDNA Library of Thermo-Photoperiod-Sensitive Genic Male Sterile (TPGMS) Wheat from Spike Developmental Stages

Large-Scale Investigation of Soybean Gene Functions by Overexpressing a Full-Length Soybean cDNA Library in Arabidopsis

Establishment and Identification of a Normalized Full-Length cDNA Library of CCRI 36

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