基于广义形态学性状对木通科的分支系统学分析

基于43个广义的形态学性状,对木通科进行了分支系统学分析。经过简约性分析,得到了68个同等简约的分支树。50％多数规则一致树的分支结构与以前建立的族划分系统基本一致。外类群大血藤属与木通科的勃奎拉藤属形成姐妹群,与以前的分支分析结果一致,但在分子系统发育树中,大血藤属却是整个木通科的姐妹群;除此之外,形态分支树的结构与分子树的结构差别不大,但一致性指数、保持性指数和各分支内部支持率均较低。单型的猫儿屎族和串果藤族位于分支树的基部,拉氏藤族与木通族是姐妹群,在木通族内,长萼木通属和木通属是姐妹群,作为一个分支;另一分支是PHS（牛藤果属、八月瓜属和野木瓜属）复合群,牛藤果属位于八月瓜属和野木瓜属各类群的基部。但八月瓜属和野木瓜属的属内系统发育关系仍有待进一步研究。     

不同品种实验兔虹膜酪氨酸酶基因序列和表达量的变化

目的从酪氨酸酶基因序列和表达量两个方面探讨酪氨酸酶与家兔虹膜颜色表型的关系。方法通过PCR扩增和测序检测4个具有不同颜色性状的家兔品种的酪氨酸酶基因外显子序列多态性;通过荧光定量PCR检测酪氨酸酶基因表达水平。结果白化品种日本大耳白兔和獭兔的TYR基因序列在第1118个碱基处都由C突变为A,并导致编码蛋白在373位,即最后一个N-糖基化位点发生由Thr到Lys的突变。白毛黑眼兔和青紫兰兔在第870个碱基处全部发生由A到T的无义突变。在白毛黑眼兔种群的所有个体和獭兔种群的部分个体中都发现TYR基因序列在第91个碱基处发生G到A的突变,导致氨基酸序列第31位处Val到Met的变异。经内参基因GAPDH的校正,TYR基因在白毛黑眼兔和青紫兰兔中表达水平显著高于在日本大耳白兔和獭兔中的表达水平（P〈0.01）。而在白毛黑眼兔和青紫兰兔之间、日本大耳白兔和獭兔之间,TYR基因的表达差异没有显著性。结论家兔TYR基因突变可能大幅度降低TYR基因表达,导致酪氨酸酶功能低下,从而影响虹膜颜色表型。     

三种豆科植物DGAT1基因家族的分子特征与进化分析

二脂酰甘油酰基转移酶广泛存在于动物、植物及酵母中,是催化三脂酰甘油生物合成的关键酶.在大豆、苜蓿和百脉草基因组中共挖掘到7个DGAT1基因,并剖析该基因的分子特征与进化关系.基因结构分析表明,3种豆科植物DGAT1基因的外显子数目变异大,其范围为3- 16.蛋白特征分析显示,3种豆科植物分享8个保守基序,同时发现2个大豆物种特有的保守基序.EST数目统计分析结果表明,该基因在3种植物的根、茎、叶、花、子叶与体细胞胚中表达,其中花器官表达量最高,EST数目占了34％.进化分析揭示了DGAT1基因是一个古老的基因家族,在植物演化历程中基因数目发生扩增现象,但其功能区仍然保持较高的保守性.     

Assembly,Target‐Signaling and Intracellular Transport of Tyrosinase Gene Family Proteins in the Initial Stage of Melanosome Biogenesis

Assembly, target‐signaling and transport of tyrosinase gene family proteins at the initial stage of melanosome biogenesis are reviewed based on our own discoveries. Melanosome biogenesis involves four stages of maturation with distinct morphological and biochemical characteristics that reflect distinct processes of the biosynthesis of structural and enzymatic proteins, subsequent structural organization and melanin deposition occurring in these particular cellular compartments. The melanosomes share many common biological properties with the lysosomes. The stage I melanosomes appear to be linked to the late endosomes. Most of melanosomal proteins are glycoproteins that should be folded or assembled correctly in the ER through interaction with calnexin, a chaperone associated with melanogenesis. These melanosomal glycoproteins are then accumulated in the trans Golgi network (TGN) and transported to the melanosomal compartment. During the formation of transport vesicles, coat proteins assemble on the cytoplasmic face of TGN to select their cargos by interacting directly or indirectly with melanosomal glycoproteins to be transported. Adapter protein‐3 (AP‐3) is important for intracellular transport of tyrosinase gene family proteins from TGN to melanosomes. Tyrosinase gene family proteins possess a di‐leucine motif in their cytoplasmic tail, to which AP‐3 appears to bind. Thus, the initial cascade of melanosome biogenesis is regulated by several factors including: 1) glycosylation of tyrosinase gene family proteins and their correct folding and assembly within ER and Golgi, and 2) supply of specific signals necessary for intracellular transport of these glycoproteins by vesicles from Golgi to melanosomes.     

Evolutionary Analysis for Functional Divergence of the Toll-Like Receptor Gene Family and Altered Functional Constraints

The Toll-like receptor (TLR) gene family consists of type 1 transmembrane receptors, which play essential roles in both innate immunity and adaptive immune response by ligand recognition and signal transduction. Using all available vertebrate TLR protein sequences, we inferred the phylogenetic tree and then characterized critical amino acid residues for functional divergence by detecting altered functional constraints after gene duplications. We found that the extracellular domain of TLR genes showed higher functional divergence than that of the cytoplasmic domain, particularly in the region between leucine-rich repeat (LRR) 10 and LRR 15 of TLR 4. Our finding supports the concept that sequence evolution in the extracellular domain may be responsible for the broad diversity of TLR ligand-binding affinity, providing a testable hypothesis for potential targets that could be verified by further experimentation.     

A heuristic method to reconstruct the history of sequences subject to recombination

Summary Sequences subject to recombination and gene conversion defy phylogenetic analysis by traditional methods since their evolutionary history cannot be adequately summarized by a tree. This study investigates ways to describe their evolutionary history and proposes a method giving a partial reconstruction of this history. Multigene families, viruses, and alleles from within populations experience recombinations/gene conversions, so the questions studied here are relevant for a large body of data and the suggested solutions should be very practical. The method employed was implemented in a program, RecPars, written in C and was used to analyze nine retroviruses.     

西红花MADS-box基因家族的生物信息学分析

西红花是中国传统中药材,以花柱入药,被誉为"植物黄金"。MADS-box转录因子家族在显花植物的花器官形成和分化过程中发挥重要作用,其有极大的可能影响西红花花器官的形成进而影响花柱发育。本研究采用生物信息学方法,对来自西红花转录组数据库中的17条MADS-box转录因子的核苷酸进行解读,及对其编码的氨基酸序列的组成成分、理化性质、信号肽、导肽、跨膜结构域、亚细胞定位、亲疏水性、蛋白质的二级、三级结构及功能域进行预测分析,并将西红花和其他植物的MADS-box蛋白进行同源比对,同时构建了西红花和模式植物拟南芥MADS-box蛋白家族的系统进化树。结果表明,西红花MADS-box基因的开放阅读框在630~750 bp左右,分子量在24~29 kD之间,理论等电点(pI)均大于7,介于8.69~9.54之间,表现为碱性疏水蛋白,既不含有信号肽也没有跨膜结构,二级结构主要原件为α-螺旋和无规则卷曲,含有一个MADS-MEF结构域和K-box结构域。氨基酸同源性比对结果表明西红花和石刁柏的MADS-box蛋白同源性较高。与拟南芥的进化树分析结果显示,西红花MADS-box蛋白可聚为两大类,分属于MIKC和Mβ亚家族。本工作可为今后进一步深入研究西红花MADS-box蛋白的生物学功能提供可靠的参考依据。     

单子叶植物科级分类阶元形态性状分支分析

基于93个形态形状,采用13个被子植物基部类群做为外类群,对49个单子叶植物科级分类阶元进行了分支系统学分析。经过简约性分析,得到了1684棵同等最大简约分支树。严格一致树的分支结构图表明：1）古草本类植物和单子叶植物是姐妹群关系;2）具有网状脉的类群,薯蓣科,菝葜科,百部科是单子叶植物的最基部类群。由于性状状态间存在着较多的平行和逆转进化,这在一定程度上影响了系统发育重建的准确性;所选择的性状状态之间的演化很可能是平行的、多次的或者是特化的状态,因此这样复杂的演化关系的探索关键在于找到一些能确切反映其系统演化关系的形态性状。目前很难通过简约化的形态分支分析来解开整个单子叶植物的起源和演化之谜。为了避开对系统学分析造成干扰的误导性状,形态数据结合DNA序列分析很可能是必需的。     

Phylogeny of Trichomonads Based On Partial Sequences of Large Subunit Rrna and On Cladistic Analysis of Morphological Data

ABSTRACT. Several domains of large subunit rRNA from nine trichomonad species have been sequenced. Molecular phylogenies obtained with parsimony and distance methods demonstrate the trichomonads are a monophyletic group which branches very early in the eukaryotic tree. the topology of the trees is in general agreement with traditional views on evolutionary and systematic relationships of trichomonads. A clear dichotomy is noted between the subfamily Trichomonadinae and the subfamily Tritrichomonadinae. In the latter subfamily, a second division separates the " Tritrichomonas muris -type" species from the " Tritrichomonas augusta -type" ones. Previous evolutionary schemes in which the Monocercomonadidae were regarded as the most "primitive" and the Trichomonadidae as more "evolved" are not in agreement with our molecular data. the emergence of Monocercomonas and Hypotrichomonas at the base of the Tritrichomonas lineage suggests a secondary loss of some cytoskeletal structures, the costa and undulating membrane in these genera. This is corroborated by the early branching position of Trichomitus. which possesses a costa and an undulating membrane and has usually been placed among the Trichomonadidae on the basis of cytological characters. A cladistic analysis was applied to the available morphological characters in order to produce a hierarchical grouping of the taxa reflecting their morphological diversity. Supplementary key words. Evolution, molecular phylogeny, morphological cladistic analysis.     

拟南芥GHMP基因家族成员的组织表达及生物信息学分析

利用生物信息学方法获得拟南芥全基因组中12个GHMP基因家族成员。通过实时定量PCR技术研究这12个基因在不同组织中的表达,结果显示它们具有组织表达特异性。构建了拟南芥中GHMP基因家族成员的系统进化树。启动子区调控元件分析表明,大多数GHMP成员包含有光响应、生物钟及其它逆境胁迫响应的相关元件,预测这些GHMP基因家族成员可能参与了植物的光信号、生物钟及相关的逆境胁迫信号转导途径。     

Evolutionary History of the 11p15 Human Mucin Gene Family

The four human mucin genes MUC6, MUC2, MUC5AC, and MUC5B are located at chromosome 11p15.5. It has been demonstrated that the three mucins MUC2, MUC5AC, and MUC5B contain several Cys-subdomains of 108 amino acid residues. In contrast, little information is available concerning MUC6. These Cys-subdomains contain 10 cysteine residues that have a highly conserved position. We present here a coherent probable evolutionary history of this human gene family after comparison of the nucleotide sequences of these Cys-subdomains. The three MUC loci MUC2, MUC5AC, and MUC5B may have evolved from a common ancestral gene by two successive duplications. Moreover, we can postulate that MUC5AC and MUC5B have evolved in a concerted manner, while MUC2 has evolved separately. Received: 30 January 1997 / Accepted: 17 April 1997     

Evolutionary Aspects of Functional and Pseudogene Members of the Phytochrome Gene Family in Scots Pine

According to the neutral theory of evolution, mutation and genetic drift are the only forces that shape unconstrained, neutral, gene evolution. Thus, pseudogenes (which often evolve neutrally) provide opportunities to obtain direct estimates of mutation rates that are not biased by selection, and gene families comprising functional and pseudogene members provide useful material for both estimating neutral mutation rates and identifying sites that appear to be under positive or negative selection pressures. Conifers could be very useful for such analyses since they have large and complex genomes. There is evidence that pseudogenes make significant contributions to the size and complexity of gene families in pines, although few studies have examined the composition and evolution of gene families in conifers. In this work, I examine the complexity and rates of mutation of the phytochrome gene family in Pinus sylvestris and show that it includes not only functional genes but also pseudogenes. As expected, the functional PHYO does not appear to have evolved neutrally, while phytochrome pseudogenes show signs of unconstrained evolution.     

Phylogeny of Plastids Based on Cladistic Analysis of Gene Loss Inferred from Complete Plastid Genome Sequences

Based on the recent hypothesis on the origin of eukaryotic phototrophs, red algae, green plants, and glaucophytes constitute the primary photosynthetic eukaryotes (whose plastids may have originated directly from a cyanobacterium-like prokaryote via primary endosymbiosis), whereas the plastids of other lineages of eukaryotic phototrophs appear to be the result of secondary or tertiary endosymbiotic events (involving a phototrophic eukaryote and a host cell). Although phylogenetic analyses using multiple plastid genes from a wide range of eukaryotic lineages have been carried out, some of the major phylogenetic relationships of plastids remain ambiguous or conflict between different phylogenetic methods used for nucleotide or amino acid substitutions. Therefore, an alternative methodology to infer the plastid phylogeny is needed. Here, we carried out a cladistic analysis of the loss of plastid genes after primary endosymbiosis using complete plastid genome sequences from a wide range of eukaryotic phototrophs. Since it is extremely unlikely that plastid genes are regained during plastid evolution, we used the irreversible Camin-Sokal model for our cladistic analysis of the loss of plastid genes. The cladistic analysis of the 274 plastid protein-coding genes resolved the 20 operational taxonomic units representing a wide range of eukaryotic lineages (including three secondary plastid-containing groups) into two large monophyletic groups with high bootstrap values: one corresponded to the red lineage and the other consisted of a large clade composed of the green lineage (green plants and Euglena) and the basal glaucophyte plastid. Although the sister relationship between the green lineage and the Glaucophyta was not resolved in recent phylogenetic studies using amino acid substitutions from multiple plastid genes, it is consistent with the rbcL gene phylogeny and with a recent phylogenetic study using multiple nuclear genes. In addition, our analysis robustly resolved the conflicting/ambiguous phylogenetic positions of secondary plastids in previous phylogenetic studies: the Euglena plastid was sister to the chlorophycean (Chlamydomonas) lineage, and the secondary plastids from the diatom (Odontiella) and cryptophyte (Guillardia) were monophyletic within the red lineage.     

繁缕核糖体失活蛋白基因克隆及序列分析

采用同源克隆结合RACE法,克隆了繁缕核糖体失活蛋白的全长cDNA,命名为q3(GenBank accession GQ870262)。序列分析结果表明,q3的开放阅读框(ORF)长780 bp,编码259个氨基酸。序列G+C含量为41.5%,与大部分Ⅰ型RIP基因相近。q3编码的蛋白质命名为Q3,理论分子量为28.16 kD,pI为9.44,均与Ⅰ型核糖体失活蛋白相近;包含由23个氨基酸组成的信号肽。功能结构域分析发现,该蛋白含有3个蛋白激酶磷酸化位点、4个络氨酸蛋白激酶磷酸化位点和7个N-肉豆蔻酰化位点。三级结构预测发现,有35.52%的氨基酸残基参与了α螺旋,24.32%的氨基酸残基组成延伸链,40.15%的氨基酸残基随机缠绕其中。基于繁缕及其近缘种核糖体失活蛋白的氨基酸序列构建的系统发育树显示,其结构与经典分类结果基本一致。     

槭树科植物广义形态学性状分支分析

通过45个广义的形态学性状对槭树科(Aceraceae)尤其是槭属(Acer L.)的主要类群做了分支分析,结果显示：1)槭属内由于各类群分布着较多的同塑性状状态,而难以为属下组间关系的解决提供更多有价值的信息;通过对具体的性状状态分布分析显示,对于象槭属这样在形态上分化较大的类群,由于多数分类性状在不同类群间经历了平行和逆转演化,因而在较低分类阶元水平很难选择合适的性状来通过分支分析构建其系统发育;2)鸡爪槭组(section Palmata)作为整个槭属的基部类群,虽然支持率较低,但与其它类群相比在槭属内维持了较多的原始性状;3)金钱槭属(Dipteronia Oliv.)的两个种作为单系得到了100％的靴带支持,且和槭属作为姐妹群也得到了较好的支持。     

乙型流感病毒河北株的HA1基因序列及种系发生的分析

对１９８９年春在河北保定分离的两株乙型流感病毒进行了抗原性、ＨＡ＿１基因序列和种系发生分析,与不同期的国内外代表株比较结果表明,自１９８８年以来乙型流感病毒变异较快,Ｂ／河北／５３／８９株的ＨＡ＿１基因序列与Ｂ／挪威／１／８５株相比,其氨基酸的同源性为９４．５２％,与同期的Ｂ／香港／２０／８９株同源性为９７．１２％。种系发生分析结果,从１９８８至１９８９年乙型流感病毒出现了５个支系,同期在保定分离的两株病毒,在同源替代中分别属于两个支系。日本国基本每隔两年出现一次乙型流感的流行优势型,其发生频度与甲型流感相似。国内少见乙型的流行优势型,可能和使用的分离病毒材料有关,日本用ＭＤＣＫ细胞比国内用鸡胚对乙型流感病毒的分离阳性率高。     

猪细小病毒SD-68株vp2基因的克隆及序列分析

对猪细小病毒(PPV)SD-68株印2基因进行的克隆和序列测定表明：SD-68株VP2基因全长1740bD,编码579个氨基酸残基组成的多肽;PPVSD-68株与Kresse株、SY-99株、NADL-2(5075)株、NADL-2(4973)株、US-1株的VP2基因比较,核苷酸的同源性在99％以上,氨基酸的同源性在96％以上。进化树分析表明SD-68株与kresse株的亲缘关系最近;在决定毒株组织嗜性的关键氨基酸位点上(378,383及436),SD-68株与kresse株的差异最小,据此推测SD-68株的组织嗜性与Kresse株相似,即SD-68株属皮炎型PPV;而比较弱毒株NADL-2、SD-68和强毒株kresse VP2的氨基酸差异后发现,215、378和383可能是决定PPV致病性强弱的关键位点。     

猪细小病毒SD-68株vp2基因的克隆及序列分析

对猪细小病毒(PPV)SD-68株vp2基因进行的克隆和序列测定表明SD-68株VP2基因全长1740bp,编码579个氨基酸残基组成的多肽;PPV SD-68株与Kresse株、SY-99株、NADL-2(5075)株、NADL-2(4973)株、US-1株的VP2基因比较,核苷酸的同源性在99%以上,氨基酸的同源性在96%以上.进化树分析表明SD-68株与kresse株的亲缘关系最近;在决定毒株组织嗜性的关键氨基酸位点上(378,383及436),SD-68株与kresse株的差异最小,据此推测SD-68株的组织嗜性与Kresse株相似,即SD-68株属皮炎型PPV;而比较弱毒株NADL-2、SD-68和强毒株kresse VP2的氨基酸差异后发现,215、378和383可能是决定PPV致病性强弱的关键位点.     

Phylogenetic Analysis of the Non-structural (NS) Gene of Influenza A Viruses Isolated in Kazakhstan in 2002-2009

Although the important role of the non-structural (NSI and NEP) gene of influenza A in virulence of the virus is well established,our knowledge about the extent of variation in the NS gene pool of influenza A viruses in their natural reservoirs in Kazakhstan is incomplete.17 influenza A viruses of different subtypes were studied in this paper.Seven types of haemagglutinin and five different neuraminidase subtypes in eight combinations were found among the isolated viruses.A comparison of nucleotide sequences of isolated viruses revealed a substantial number of silent mutations,which results in high degree of homology in amino acid sequences.By phylogenetic analysis it was shown that two distinct gene pools,corresponding to both NS allele A with 5 Clades and B,were present at the same time in Kazakhstan.The degree of variation within the alleles was very low.In our study allele A viruses had a maximum of 5％ amino acid divergence in Clade while allele B viruses had only 4％ amino acid divergence.