植物异源多倍体进化中基因表达的变化

多倍化是植物物种进化的主要动力,异源多倍体植物在形成早期发生着快速的基因表达变化。本文概述了异源多倍体植物中基因表达变化的特点,包括基因的沉默、激活和部分同源基因表达水平的变化,探讨了基因表达变化的分子机制和生物学意义,并对研究中的问题进行了分析和展望。     

山羊草属异源多倍体植物基因组进化的ISSR分析

使用31个ISSR引物对山羊草属Aegilops多倍体植物及其祖先二倍体（共23种）的基因组进行了分析,结果表明：与其二倍体祖先种相比,异源多倍体物种的基因组发生了很大变化。在含U基因组的异源多倍体物种中,U基因组相对而言变化很小,而其他基因组则发生了不同程度的变化。这表明当U基因组与其他基因组共存于多倍体物种中时,U基因组表现出较强的“同化效应”。对这些基因组的进化进行了讨论。     

低拷贝核基因在异源多倍体植物中的进化与表达

异源多倍体植物在自然界中广泛分布。在这类植物谱系中, 低拷贝核基因具有特殊的进化特点和丰富的植物系统发生信息, 在转录水平存在基因沉默、基因激活和不均等表达等特点。以低拷贝核基因为主线, 概述了其在多倍体植物系统发生中的应用和相关注意事项, 并对其在多倍体植物中的表达变化及其分子机制进行了探讨, 系统地介绍了国际上相关领域的研究成果和最新动向。     

植物多倍体化中基因组和基因表达的变化

多倍体化在植物进化的历史过程中频繁发生, 对新物种的形成产生了很大影响。伴随着多倍体化, 植物在基因组和基因表达上发生了复杂的变化, 包括染色体数目变化、染色体重组、基因沉默、基因的非加性表达和表观遗传等变化。该文对多倍体化引起的这些变化及其相应的机理进行了综述, 以期为了解多倍体化中植物新表型的产生机理和在进化中的意义提供参考。     

黄瓜属不同倍性异源多倍体的形态及生理特性分析

以黄瓜属3种不同倍性异源多倍体为试验材料,比较分析它们的形态和生理特性与基因组剂量的关系,为进一步研究黄瓜属基因组剂量效应、探讨植物多倍体进化机理奠定基础。结果表明:(1)黄瓜属异源四倍体与种间杂种F1相比,其叶片厚度、主蔓直径等性状随基因组剂量的增加而增大,而果实大小、主蔓节间长以及果瘤果刺的大小随基因组剂量的增加而减小。(2)在异源三倍体中,叶片厚度和主蔓直径等表型性状也表现出一定的基因组剂量效应。(3)基因组剂量的变化会引起黄瓜属异源多倍体中叶绿素含量、POD活性以及IAAi、PA和ZR等内源激素的变化。     

远缘杂交早代稳定小麦导入了外源DNA片段并发生了DNA重排

在植物界, 多倍体植物非常普遍. 具有A, B, D三个部分同源染色体组的普通小麦是异源多倍体物种的一个典型代表. 近几年, 模拟普通小麦的起源过程进行的研究表明, 从四倍体小麦注入节节麦整个基因组形成异源六倍体小麦的早期阶段, DNA序列和基因表达发生了可能有利于遗传“二倍化”的变化. 利用普通小麦-黑麦远缘杂交自然结实的早代稳定特异小麦99L2研究发现: (ⅰ) 99L2至少导入了两个黑麦染色体上的DNA片段, 表明可能存在不同于传统的小麦-外源染色体配对重组的外源DNA导入机制; (ⅱ) 99L2自身的DNA序列发生了变化, 表明外源DNA部分片段注入小麦染色体组过程中, 也可能导致小麦自身DNA序列发生变化.     

多倍体植物抗逆性研究进展

许多逆境能诱导多倍体植物发生,并可能作为筛选压力推动多倍体的形成。多倍体植物具有细胞、器官巨大化的特点,但株型不一定巨大化。在几种主要逆境条件下(如低温、高温、干旱、盐碱、病害等),多倍体植物抗逆性往往增强。多倍体植物主要通过调整细胞大小和结构、调节生物膜系统、提高渗透调节物质含量、增强抗氧化系统活性、增加基因表达和通过表观遗传变化来增强抗逆性,但也有研究显示多倍体植物的抗逆性降低。多倍体植物的抗逆性还需要更深入和细致研究,才能阐明抗逆机理。该文对近年来国内外有关多倍体植物的形成、特征、抗逆性表现及其调控机制等方面的研究进展进行综述。     

异源多倍体植物核rDNA序列的同步进化

同步进化是异源多倍体植物核rDNA序列进化的重要方式,同步进化的程度在不同植物类群中存在较大差异,有些类群中同步进化力量较强,核rDNA重复序列间已经纯合或接近纯合,有些类群中同步进化的力量较弱,可观察到序列的杂合性。同步进化的机制主要是不等交换和基因转换,并受异源多倍体形成年代、生殖方式、基因突变率等因素的影响。     

多倍体植物的表观遗传现象

表观遗传现象是指基因表达发生改变但不涉及DNA序列的变化, 它存在于许多植物的多倍体化过程中,而且能够在代与代之间传递。表观遗传变异包括基因沉默、DNA甲基化、核仁显性、休眠转座子激活和基因组印记等方面。这种现象可能是由于基因组间的相互作用直接诱发基因沉默或基因表达改变所致;也可能由DNA甲基化之外的组蛋白编码的改变引起;或者与甲基化不足、染色质重组或转座子激活等有关。表观遗传变异在提高基因表达的多样性,引起遗传学和细胞学上的二倍化,以及促进基因组间的相互协调等方面起着重要作用。文章综述了植物多倍体化过程中的表观遗传现象及其在多倍体植物基因组进化中的作用,并在此基础上提出了今后在这方面的研究途径。     

稻属多倍体的研究历史及存在问题

稻属Oryza隶属于禾本科Poaceae稻亚科Oryzoideae稻族Oryzeae, 包括20多个种, 其中近1/2的种类为异源多倍体植物。这些多倍体不但数量多而且涉及BC、CD、HJ和HK等多种染色体组构成, 广泛分布于热带亚洲、非洲、大洋洲和拉丁美洲。由于具有重要的经济和理论研究价值, 稻属植物一直在植物学研究中备受瞩目。相应地, 稻属多倍体植物的研究也积累了丰富的资料。本文通过回顾以往对稻属植物的研究历史, 特别关注有关多倍体的研究, 结合我们最近的研究总结了稻属多倍体分类和系统发育关系研究的最新进展, 同时对稻属多倍体研究中存在的问题及未来研究方向进行了讨论。     

Evolution of duplicate gene expression in polyploid and hybrid plants

Allopolyploidy is a prominent mode of speciation in flowering plants. On allopolyploidy, genomic changes can take place, including chromosomal rearrangement and changes in gene expression; these processes continue over evolutionary time. Recent studies of gene expression in polyploid and hybrid plants, reviewed here, have examined expression in natural polyploids and synthetic neopolyploids as well as in diploid and F(1) hybrids. Considerable changes in gene expression have been observed in allopolyploids, including up- or downregulation of expression in the polyploids compared with their parents, unequal expression of duplicated genes, and silencing of one copy. Genes in a variety of functional categories show altered expression, and the patterns vary considerably by gene. Some changes seem to be stochastic, whereas others are repeatable. Gene expression changes can be organ specific. Reciprocal silencing of duplicates in different organs has been observed, suggesting subfunctionalization and long-term retention of duplicates. It has become clear that hybridization has a much greater effect than chromosome doubling on gene expression in allopolyploids. Diploid and triploid F(1) hybrids can show alterations of expression levels compared with their parents. Parent-of-origin effects on gene expression have been examined, and loss of gene imprinting has been shown. Some gene expression changes in polyploids and hybrids can be correlated with phenotypic effects. Demonstrated mechanisms of gene expression changes include DNA methylation, histone modifications, and antisense RNA. Several hypotheses have been proposed for why gene expression is altered in allopolyploids and hybrids.     

多倍体植物中基因表达模式的变化

植物杂交和多倍化能导致基因组结构发生变化,并显著影响了基因表达,因此认为杂交和多倍化是促进植物进化的一个重要力量。近些年大量的研究表明植物多倍化后基因表达模式发生了复杂的改变,包括基因沉默、基因表达的基因组偏向性及组织特异性、基因激活等现象,本文对这些现象及其特点和机制进行了综述。     

Evaluating the role of natural selection in the evolution of gene regulation

Surveys of gene expression reveal extensive variability both within and between a wide range of species. Compelling cases have been made for adaptive changes in gene regulation, but the proportion of expression divergence attributable to natural selection remains unclear. Distinguishing adaptive changes driven by positive selection from neutral divergence resulting from mutation and genetic drift is critical for understanding the evolution of gene expression. Here, we review the various methods that have been used to test for signs of selection in genomic expression data. We also discuss properties of regulatory systems relevant to neutral models of gene expression. Despite some potential caveats, published studies provide considerable evidence for adaptive changes in gene expression. Future challenges for studies of regulatory evolution will be to quantify the frequency of adaptive changes, identify the genetic basis of expression divergence and associate changes in gene expression with specific organismal phenotypes.     

Evolution of yellow gene regulation and pigmentation in Drosophila

BACKGROUND: Changes in developmental gene expression are central to phenotypic evolution, but the genetic mechanisms underlying these changes are not well understood. Interspecific differences in gene expression can arise from evolutionary changes in cis-regulatory DNA and/or in the expression of trans-acting regulatory proteins, but few case studies have distinguished between these mechanisms. Here, we compare the regulation of the yellow gene, which is required for melanization, among distantly related Drosophila species with different pigment patterns and determine the phenotypic effects of divergent Yellow expression. RESULTS: Yellow expression has diverged among D. melanogaster, D. subobscura, and D. virilis and, in all cases, correlates with the distribution of black melanin. Species-specific Yellow expression patterns were retained in D. melanogaster transformants carrying the D. subobscura and D. virilis yellow genes, indicating that sequence evolution within the yellow gene underlies the divergence of Yellow expression. Evolutionary changes in the activity of orthologous cis-regulatory elements are responsible for differences in abdominal Yellow expression; however, cis-regulatory element evolution is not the sole cause of divergent Yellow expression patterns. Transformation of the D. melanogaster yellow gene into D. virilis altered its expression pattern, indicating that trans-acting factors that regulate the D. melanogaster yellow gene have also diverged between these two species. Finally, we found that the phenotypic effects of evolutionary changes in Yellow expression depend on epistatic interactions with other genes. CONCLUSIONS: Evolutionary changes in Yellow expression correlate with divergent melanin patterns and are a result of evolution in both cis- and trans-regulation. These changes were likely necessary for the divergence of pigmentation, but evolutionary changes in other genes were also required.     

Temporal analysis of gene expression in a field population of the Scleractinian coral Montastraea faveolata

Organisms maintain homeostasis and abate cellular damage by altering gene expression. Coral colonies have been shown to produce unique gene expression patterns in response to different environmental stimuli. In order to understand these induced changes, the natural variation in expression of genetic biomarkers needs to be determined. In this study, an array of genes isolated from Scleractinian coral was used to track changes in gene expression within a population of Montastraea faveolata from April to October 2001 in the Florida Keys. The profiles of genes observed in this study can be divided into two groups based on expression over this time period. In spring and early summer, May through July, most of the genes show little deviation from their average level of expression. In August and September, several genes show large deviations from their average level of expression. The physiological and environmental triggers for the observed changes in gene expression have not yet been identified, but the results show that our coral stress gene array can be used to track temporal changes in gene expression in a natural coral population.     

In vitro analysis of integrated global high-resolution DNA methylation profiling with genomic imbalance and gene expression in osteosarcoma

Genetic and epigenetic changes contribute to deregulation of gene expression and development of human cancer. Changes in DNA methylation are key epigenetic factors regulating gene expression and genomic stability. Recent progress in microarray technologies resulted in developments of high resolution platforms for profiling of genetic, epigenetic and gene expression changes. OS is a pediatric bone tumor with characteristically high level of numerical and structural chromosomal changes. Furthermore, little is known about DNA methylation changes in OS. Our objective was to develop an integrative approach for analysis of high-resolution epigenomic, genomic, and gene expression profiles in order to identify functional epi/genomic differences between OS cell lines and normal human osteoblasts. A combination of Affymetrix Promoter Tilling Arrays for DNA methylation, Agilent array-CGH platform for genomic imbalance and Affymetrix Gene 1.0 platform for gene expression analysis was used. As a result, an integrative high-resolution approach for interrogation of genome-wide tumour-specific changes in DNA methylation was developed. This approach was used to provide the first genomic DNA methylation maps, and to identify and validate genes with aberrant DNA methylation in OS cell lines. This first integrative analysis of global cancer-related changes in DNA methylation, genomic imbalance, and gene expression has provided comprehensive evidence of the cumulative roles of epigenetic and genetic mechanisms in deregulation of gene expression networks.     

Hepcidin and hemojuvelin gene expression in rat liver damage: in vivo and in vitro studies

In this work, we used two rat models, partial hepatectomy (PH) and CCl(4) administration, to study the changes in iron pathways in response to hepatic damage. Liver injury induced changes in the hepatic gene expression of hepcidin, hemojuvelin (Hjv), several other proteins of iron metabolism, and several cytokines such as IL-1beta, IL-6, TNF-alpha, and IFN-gamma. Hepcidin gene expression was upregulated between 4 and 8 h with a maximum up to 16 h after surgery. However, Hjv gene expression was downregulated at the same time. An early upregulation of hepcidin (3 h) and downregulation of Hjv gene expression was found after CCl(4) administration. Transferrin receptor 1 and ferritin H gene expression was upregulated, whereas ferroportin 1 gene expression was downregulated. Hepatic IL-6 gene expression was upregulated early after PH and reached maximum 8 h after the PH. In CCl(4)-induced liver injury, IL-6, IL-1beta, TNF-alpha, and IFN-gamma upregulation were found at the maximum 12 h after the administration of the toxin. Treatment of isolated rat hepatocytes with IL-6 and, to a lesser extent, with IL-1beta but not with TNF-alpha or IFN-gamma dose dependently upregulated hepcidin and downregulated Hjv gene expression. In hepatic damage, changes of the hepatic gene expression of the main proteins involved in iron metabolism may be induced by locally synthesized mediators.