摘要
忽地笑Raised Secondary Lateral Veins(RSLV)突变体平行脉间横向二级侧脉显著凸起,生长不良,雄蕊完全退化。本研究利用表达型噬菌体载体ZAP构建了野生型和突变体忽地笑叶片cDNA文库,分别随机挑取cDNA克隆进行5′端测序,共得到3,122条有效ESTs。利用这些ESTs序列,选择非冗余基因,设计512条70mer的特异性序列为寡核苷酸探针,制作芯片,对忽地笑野生型和突变体叶器官进行基因表达谱分析。进一步采用实时定量PCR技术验证芯片实验结果,最终确定所检测的基因中,有5个基因在突变型和野生型间表达差异显著,分别是韧皮部蛋白2(phloem protein2,PP2)、铁蛋白(ferritin)、果胶甲酯酶(pectin methyl esterases,PMEs),以及叶绿素a/b结合蛋白和丙酮酸脱羧酶等。克隆获得了其全长cDNA,并探讨了这些差异基因与忽地笑突变型形成的可能关系。
Lycoris aurea exhibits parallel venation, the main vein with many lateral veins in a longitudinal parallel arrangement. There are secondary lateral veins (SLV) between each longitudinal veins. In general, SLVs are not remarkable. In this paper, the material was one kind of Lycoris aurea mutant called Raised Secondary Lateral Veins mutant (RSLV), because many Raised Secondary Lateral Veins are in abaxial surface of its leaves. Its growing potential is weaker than that of wild type and its blades are very thin. Moreover, the stamens of RSLV degenerate completely. Two cDNA libraries were constructed from RSLV mutant and wild type (WT) leaves. From the libraries, 3,122 ESTs, which are longer than 100 bp each after vector sequence removed, were acquired by single-pass sequencing from the 5' end. Following a multistep selection, 512 70-mer oligo-DNA probes were designed for attachment on the microarray slide based on the ESTs. The gene expression profile of RSLV mutant and WT leaves was compared through the microarray at transcriptional level. The microarray experiment results were further confirmed by Quantitative Real-Time PCR (QRT-PCR). We identified 5 genes whose expressions changed more than 2-fold between RSLV mutant and WT leaves. They encode phloem protein 2 (PP2), ferritin, pectin methyl esterase (PME), chlorophyll a/b binding protein (CAB protein) and pyruvate decarboxylase (PDC), respectively. Furthermore, the full-length cDNA sequences of the 5 genes were separately obtained from RSLV and WT by RACE. The relationship between differential expressions of the genes and the formation of the RSLV mutant phenotype were discussed.
出处
《遗传》
CAS
CSCD
北大核心
2007年第4期490-498,共9页
Hereditas(Beijing)
基金
科技部"863"项目(编号:2002AA241051)~~
