新疆3种雅罗鱼线粒体DNA细胞色素b序列的差异与系统进化

利用鲤科鱼类线粒体DNA细胞色素b通用引物对分布在新疆的准噶尔雅罗鱼(Leuciscusmerzbacheri)、贝加尔雅罗鱼(L .baicalensis)和高体雅罗鱼(L .idus) 3个鱼种共1 5尾个体的线粒体DNACytb部分核苷酸序列进行了测定,获得1 5条长度为41 3bp的同源基因序列。同源基因序列分析显示,在3种雅罗鱼1 5条mtDNACytb基因片段中,A、T、C、G碱基的平均含量分别是:2 7 4%、2 6 7%、1 7 2 %、2 8 7% ,其中A T含量(5 4 1 % )高于G C含量(4 5 9% ) ;共检测到5 2个突变位点;转换比颠换发生频率高,转换颠换比值(R)是3 5。mtDNACytb的进化速率在3种雅罗鱼间表现出不一致性,贝加尔与高体雅罗鱼、贝加尔与准噶尔雅罗鱼种间遗传距离分别是0 1 2 5 1和0 1 2 61 ,保守性较低;高体与准噶尔雅罗鱼种间的遗传距离是0 0 0 0 7,高度保守。mtDNACytb分子系统树显示,在3种雅罗鱼中贝加尔雅罗鱼独立成一枝,高体雅罗鱼和准噶尔雅罗鱼聚成一类。提示了,在mtDNACytb分子水平上,高体雅罗鱼和准噶尔雅罗鱼的亲缘关系十分相近,贝加尔雅罗鱼与准噶尔雅罗鱼的亲缘关系相距较远。我们对准噶尔、贝加尔和高体雅罗鱼mtDNACytb方面的研究与陈星玉对其骨骼类型的研究结果相吻合。     

准噶尔雅罗鱼β-肌动蛋白基因启动子的克隆及其活性功能初步检测

以开发利用新疆濒危鱼类准噶尔雅罗鱼(Leuciscus merzbacheri)基因资源为研究目的, 利用PCR技术克隆准噶尔雅罗鱼的β-actin 基因, 得到的β-actin 基因片段SZ21包含启动调控区, 大小为2 398 bp。SZ21的启动调控区包括β-actin 基因上游调控序列、第1、第2、第3和第4外显子部分序列。上游调控序列中含有对转录起重要作用的CAAT框、TATA 框和CArG 框等元件。对启动子序列在线分析表明, 获得的启动子含有E-box、RU49、ZBPF、CEBP、CREB等多个重要转录因子结合位点。用AatⅡ破坏真核表达载体pEGFP-N1-AFPⅢ中的CMV启动子, 将准噶尔雅罗鱼的SZ21启动调控区克隆到载体pEGFP-N1-AFPⅢ(CMV坏)上, 构建成重组表达载体β2 pEGFP-N1-AFPⅢ。脂质体转染BHK-21细胞。结果表明, 克隆的准噶尔雅罗鱼β-actin基因启动子SZ21具有启动EGFP报告基因在哺乳动物细胞中表达的活性。通过BHK-21绿色荧光细胞的传代证实, 克隆的启动子具有持续启动蛋白基因表达的活性, 在细胞传代中可以遗传。PCR检测传代的BHK-21绿色荧光细胞基因组DNA, 均能检测到SZ21目的片段。文章成功分离了具有活性功能的准噶尔雅罗鱼β-actin基因启动子。     

准噶尔雅罗鱼β-肌动蛋白基因启动子克隆及序列分析

利用PCR方法克隆了准噶尔雅罗鱼(Leuciscus merzbacheri)的β-actin基因启动子片段SZ21,大小是2398bp。对克隆的启动子序列进行了转录调控元件的生物信息学预测分析,同时,基于启动子中包含的开放阅读框和内含子序列,探讨了准噶尔雅罗鱼与鲤鱼(Cyprinus carpio)、草鱼(Ctenopharyngodon idella)、青鱼(Mylopharyngodon piceus)、团头鲂(Megalobrama amblycephala)、泥鳅(Misgurnus mizolepis)间的系统进化关系。结果显示,该启动子序列的3个核心启动子转录元件:CAAT-box、CArGmotif和TATA-box分别在转录起始位点(+1)上游的-89、-59、-26处,序列中还含有MEF2、SATB、CHRF、INRE、MTEN、E-box、RU49、ZBPF、CREB、Enhance region、CEBP位点等多种转录调控元件。在剪接体内含子中,剪接位点遵循GT…AG法则。启动子SZ21序列含有3个内含子和155个氨基酸。内含子1、内含子2、内含子3的系统发育分析表明,团头鲂与草鱼和青鱼的亲缘关系要比与准噶尔雅罗鱼的更近一些,这与传统分类中的亲缘关系显示不一致,其原因尚需探讨。     

新疆3种雅罗鱼线粒体DNA控制区序列的差异和系统进化关系

对分布在新疆的准噶尔雅罗鱼(Leuciscus merzbacheri)、贝加尔雅罗鱼(Leuciscus leuciscus baicalensis)和高体雅罗鱼(Leuciscus idus)3个鱼种共24尾个体的线粒体DNA D-loop控制区核苷酸序列进行了测定,获得24条长度为667—669bp的同源基因序列。3种雅罗鱼之间的序列差异在6．39％—9．89％之间,贝加尔雅罗鱼与高体雅罗鱼种间序列同源性高,变异程度小;贝加尔雅罗鱼与准噶尔雅罗鱼种间序列同源性最低,变异程度最大。所采集的贝加尔雅罗鱼两个地理群体(赛里木湖和额尔齐斯河)内mtDNA的平均核苷酸碱基序列差异为1．07％和1．08％;两群体间的序列差异为1．07％,显示两个地理群体间无明显分化。DNA序列数据显示,这3种鱼类线粒体DNAD-loop序列变异丰富,24尾个体呈现独自的单倍型。同源基因序列平均含AT碱基64．1％,GC碱基35．9％,显示准噶尔雅罗鱼、贝加尔雅罗鱼、高体雅罗鱼的线粒体DNAD-loop区核苷酸组成的不均一性。分子系统树提示,贝加尔雅罗鱼与高体雅罗鱼亲缘关系较近,准噶尔雅罗鱼是3种雅罗鱼中较古老的鱼种。     

新疆三种雅罗鱼属鱼类mtDNA D-loop多态性及起源分化分析

用PCR-RFLP技术,对新疆分布的准噶尔雅罗鱼、贝加尔雅罗鱼和高体雅罗鱼的mtDNA D-loop高变区约827bp进行了扩增,用ScaI、HinfI、AluI、DdeI 4种限制性内切核酸酶对56个样本的扩增产物酶切和RFLP分析,共检测到6种单倍型。准噶尔雅罗鱼存在2种单倍型：BDAA和BDBA;贝加尔雅罗鱼存在3种：AAAA、ABAA和ACAA;高体雅罗鱼只有1种。初步认为,准噶尔雅罗鱼、贝加尔雅罗鱼存在较丰富的群体内变异。用6种单倍型及净遗传距离绘制的UPGMA分子系统树,提示准噶尔雅罗鱼有可能是原始种,贝加尔雅罗鱼和高体雅罗鱼是由准噶尔雅罗鱼进化而来。 Abstract:PCR-RFLP technique was employed to amplify about 827bp of mtDNA D-loop hypervariable region of Leuciscus baicalensis,L.merzbacheri and L.idus in Xinjiang.The PCR products of 56 samples with four restriction enzymes were digested:ScaI,HinfI,AluI,DdeI,and RFLP analysis was done then.The study indicates that all of L. species and populations have six haplotypes,L.merzbacheri has two haplotypes:BDAA,BDBA;L.baicalensis has three:AAAA,ABAA,ACAA;L.idus has one:CAAA.It is primarily considered that L.merzbacheri and L.baicalensis have more intra-population mutations.The UPGMA trees with 6 haplotypes and net genetics distance pointed out that L.merzbacheri might be original species,L.baicalensis and L.idus are evolved from L.merzbacheri.     

准噶尔雅罗鱼染色体核型及带型的初步研究

以肾细胞作材料,采用秋水仙素-低渗-空气干燥法、Ag-NORs、C-带和G-带显带技术对准噶尔雅罗鱼(Leuciscus merzbacheri)染色体进行了研究。结果表明:(1)准噶尔雅罗鱼2n=50,核型组成为18m+14sm+6st+12t,NF=82,没有异型性染色体分化。(2)Ag-NORs的数目在不同的细胞中表现出多态性,数目为1～2个,出现1个Ag-NORs的频率最低(10%),出现2个的频率最高(70%);Ag-NORs主要出现在m1对和m4对同源染色体上;未发现有Ag-NORs联合的现象。(3)准噶尔雅罗鱼的染色体均呈现C-带阳性,可分为着丝粒C-带和端粒C-带。(4)同源染色体上G-带带纹基本一致,其带纹在每对染色体上的数目及分布具有明显特征性。     

近交系剑尾鱼的遗传生化标记研究

目的通过研究对RR-B、RW-H、BY-F三个近交系和非选育剑尾鱼的研究比较,建立近交系剑尾鱼的遗传生化标记检测技术。方法依照国标GB／T14927.1-2008的遗传操作规程优化实验条件,对三个近交品系及非选育群剑尾鱼的不同组织的6个遗传生化位点进行研究,以得到其遗传生化图谱。结果在6个生化位点中,同一品系剑尾鱼同工酶存在组织特异性,多数同工酶在肝中活性较强。同一生化位点在不同品系间存在差异。RR-B系在葡萄糖磷酸异构酶（Gpi）、6-磷酸葡萄糖脱氢酶（Gpd）位点表现出特异性条带,RW-H系在过氧化氢酶（Ce）位点表现出特异性条带。同一生化位点在各品系内表现较为一致,而在非选育剑尾鱼中在上述三个生化位点表现出多态性。在酯酶（ES）、碱性磷酸酶（AKP）、乳酸脱氢酶（LDH）位点,各品系谱带不易区分其差异。结论建立了剑尾鱼近交系生化标记检测技术,可望用于近交系剑尾鱼的遗传质量监测。     

北太平洋柔鱼微卫星标记的筛选及遗传多样性

采用(AC)12、(AG)12两种生物素探针,通过磁珠富集法构建了柔鱼部分基因组微卫星富集文库。68个阳性克隆中有60个含有微卫星序列,重复次数在10次以上的占86.84%,最高重复次数为33次。其中,完美型微卫星占60.53%,非完美型微卫星占36.84%,混合型微卫星占2.63%。除探针使用的AC/TG、AG/TC重复外,还得到ACAG、AGAC重复序列。利用筛选出的8个微卫星位点对北太平洋柔鱼6个群体的遗传多样性及遗传结构进行分析。结果表明,8个微卫星位点均为高度多态性位点(PIC=0.787—0.987),位点Bo103与位点Bo105极显著偏离Hardy-Weinberg平衡(P0.01)。6个地理位置的柔鱼群体显示出较高的遗传多样性水平(Ho=0.672—0.761,He=0.808—0.851)。两两群体间的Fst值以及AMOVA分析结果均表明,群体间遗传分化不显著(Fst=0.00559,P0.05),遗传差异主要来自于个体间。基于Nei's遗传距离的UPGMA聚类树显示,北太平洋东北部2个柔鱼群体(NE1、NE3)聚为一类,西北部3个群体(NW1、NW2、NW3)与东北部1个群体(NE2)另聚为一类,且群体NW1与群体NE2亲缘关系最近,遗传距离与地理距离线性相关分析没有呈现出正相关性(R=0.175,P0.05)。遗传结构分析结果推断北太平洋柔鱼存在1个理论群。柔鱼个体具有较强的游泳能力,在海流的作用下,群体之间存在较强的基因交流。建议今后在柔鱼资源开发利用过程中将北太平洋柔鱼看作1个管理单元。     

高原鼢鼠肝脏组织细胞周期相关基因的进化和表达

高原鼢鼠Myospalax baileyi是一种世居青藏高原的地下鼠,对严重的低氧环境有很强的适应性。低氧诱导细胞周期G1、G2期阻滞。为了探讨高原鼢鼠适应低氧环境的分子机制,应用生物信息学方法对p53下游细胞周期基因p21、CyclinD1、CyclinE、CDK6、CDK2、14-3-3-σ、Gadd45α、B99和CyclinB1的序列和编码的氨基酸序列进行了进化分析,并以SD大鼠Rattus norvegicus为对照,研究了这些基因在不同海拔(3300 m、2260 m)条件下的表达模式。结果表明:(1)高原鼢鼠细胞周期相关基因的序列与以色列鼹鼠Nannospalax galili同源性最高,达到90%以上;p21、CyclinD1、CyclinE和CyclinB1编码蛋白与以色列鼹鼠存在明显的趋同进化位点;SIFT评估发现,p21和CyclinB1氨基酸序列分别在第27号位点和第105号位点的变异对细胞周期调控功能有显著影响;(2)与低海拔条件相比,在高海拔条件下,高原鼢鼠肝脏组织中与G1期相关的基因p21表达水平显著上升,p21下游基因CyclinD1、CyclinE、CDK6和CDK2表达水平显著下降,而在SD大鼠中没有显著变化;与G2期相关的基因Gadd45α、B99、14-3-3-δ和CyclinB1在高原鼢鼠和SD大鼠中随海拔变化不发生明显变化。在不同海拔条件下,高原鼢鼠肝脏组织中的上述细胞周期相关基因的表达水平均极显著高于SD大鼠(P<0.01)。以上结果提示,高原鼢鼠经过长期的低氧适应,通过上调p21基因的表达抑制下游CyclinD1、CyclinE、CDK6和CDK2基因的表达,导致细胞周期G1期阻滞,从而提供充足的时间进行DNA修复,保证了DNA复制的准确性;同时高原鼢鼠肝脏组织中细胞周期的调控不仅与细胞周期基因的表达水平有关,而且可能与细胞周期因子p21的第27号位点和CyclinB1的第105号位点的变异有关。     

团头鲂的胚胎及成体组织中八种同工酶系统的研究

用垂直的淀粉凝胶电泳方法分析了胚胎发育阶段(0—105小时)和成体6种组织中的乳酸脱氢酶(LDH)、苹果酸脱氢酶(MDH)、谷氨酸脱氢酶(GDH)、葡萄糖—6—磷酸脱氢酶(G6PD)、醇脱氢酶(ADH)、异柠檬酸脱氢酶(IDH)、酯酶(EST)和碱性磷酸酶(AKP)等8种同工酶系统的酶带。共约有23个基因座位在其胚胎发育期和成体组织中表达。所分析的大多数同工酶在团头鲂个体发生过程中表达的情况大致可分为3种类型：①胚胎发育期间持续存在的同工酶类,它们在成体组织中无特异性分布;②到胚胎发育后期才开始表达的同工酶类,它们往往和特定的组织或器官的形态发生或机能分化紧密相关,并在成体组织中呈特异性分布;③在成体组织中都没有被发现而只在胚胎发育期所特有的同工酶。团头鲂的MDH同工酶类之间以及它们和G6PD同工酶活性变化之间存在着相关性,二者可能存在共同的调控机制。与许多其他鱼类不同,团头鲂的GDH同工酶在整个胚胎发育过程中都有活性,但在其成体组织中无特异性分布。基因调控系统的时空精确性是保证团头鲂胚胎发育正常代谢活动的必要条件。     

Inheritance and linkage relationships of ten isozyme genes in hazelnut

Summary The inheritance of 6-phosphogluconate dehydrogenase (6PGD), malate dehydrogenase (MHD), aconitase (ACO), phosphoglucomutase (PGM), phosphoglucoisomerase (PGI), and glutamate-oxalacetate transaminase (GOT) polymorphic isozymes was studied in leaf extracts of nine hazelnut progenies using horizontal starch gel electrophoresis. Evidence of Mendelian inheritance was obtained for ten loci: 6-Pgd-2, Mdh-1, Aco-1, Aco-2, Pgm-1, Pgm-2, Pgm-3, Pgi-2, Pgi-3, and Got-2, which permitted the analysis of 28 alleles (2.8 per locus). The presence of null alleles was detected in Pgm-1 and Pgm-3. Joint segregation analysis of pairs of isozymes revealed four linkages: Mdh-1-Pgi-2, Aco-2-Pgm-2, Pgm-1-Pgm-3, and 6Pdg-2-Pgm-2.     

Electrophoretic variation at flight-related enzyme loci and its possible association with flight capacity inEpiphyas postvittana

Variations at three flight-related enzyme loci, -glycerophosphate dehydrogenase (-Gpdh), glucose-6-phosphate dehydrogenase (G6pd), and phosphoglucomutase (Pgm), ofEpiphyas postvittana (Walker) moths were investigated using starch gel electrophoresis. Among the three enzyme loci, -Gpdh andG6pd were found to be monomorphic, butPgm was polymorphic, with a total of seven different genotypes and five alleles identified in this study. Comparisons of allozyme variability at thePgm locus showed significant differentiation among five natural populations sampled from geographically distinct localities in New Zealand and Australia and between laboratory populations differentiated by artificial selection on flight capacity. ThePgm polymorphism was shown to be associated with the variation of flight capacity, but the role of the enzyme locus in the evolution of flight behavior is to be demonstrated in this species.This work was supported by the research scholarship of the University of New England.     

Genetics of α-amylases from rye endosperm

Summary Fifteen inbred lines of rye, F₁ and F₂ progenies from crosses between lines were studied using polyacrylamide gel electrophoresis. Conventional genetic analysis of -amylase zymograms showed that the 19 bands detected in the endosperm of germinating caryopses were controlled by three linked structural loci and one independent modifying locus, which influenced the electrophoretic mobility of isozymes. Two codominant alleles were found at the -Amy1, -Amy2 structural loci and the M--Amy modifying locus while the -Amy3 locus had three alleles. Double-banded expression of the -amylase alleles was probably due to the simultaneous presence of modified and unmodified forms of isozymes on the zymogram.This work was supported by Polish Academy of Sciences under project MR-II/7 and was also a part of the author's PhD Thesis     

Duplicated phosphoglucose isomerase genes in avocado

Summary Avocado (Persea americana) cultivars were assayed for phosphoglucose isomerase (PGI) isozymes using starch gel electrophoresis. Three PGI genes were identified: one monomorphic locus, Pgi-I, coding for the plastid isozyme and two independently assorting loci, Pgi-2 and Pgi-3, coding for the cytosolic isozymes. The genetic analysis was based on comparisons of PGI zymograms from somatic and pollen tissue and on Mendelian analysis of progeny from selfed trees. The isozymic variability for PGI can be used for cultivar identification and for differentiating between hybrid and selfed progeny in avocado breeding.     

Genetic Diversity and Divergence in Chinese Yak (Bos grunniens) Populations Inferred from Blood Protein Electrophoresis

In 6 Chinese yak (Bos. Grunniens) populations including 177 yaks, 34 blood protein loci were studied by horizontal starch gel electrophoresis, four of these loci (AKP, ALB, LDH-1, TF) were found to be polymorphic. The percentage of polymorphic loci(P) is 0.118, the mean individual heterozygosity(H) is 0.015, which means a low level of genetic diversity in the whole Chinese yak population. The coefficient of gene differentiation (G _ST ) is 0.0625, which indicated an almost-indistinguishable divergence among different populations at the level of blood protein electrophoresis.     

Dissociation-recombination of intergenic sunflower alcohol dehydrogenase isozymes and relative isozyme activities

Two unlinked genes, Adh ₁ and Adh ₂, control the production of alcohol dehydrogenase (ADH) in seeds of the annual sunflower (Helianthus annuus). Each gene is polymorphic, having F and S alleles. Starch gel electrophoretic zymograms of the four possible double homozygotes have three bands, representing two homodimers and an intermediately migrating intergenic isozyme. Zymograms of double heterozygotes consist of nine bands produced by ten isozymes: six intragenics and four intergenics, two of which are coincident. Results of dissociation-recombination (D-R) experiments are reported which demonstrate the subunit composition of the intergenic isozymes, thus supporting the relationships suggested by genetic studies. Densitometric tracings of the zymogram of a cleared gel and measurements of activities of homodimer isozymes eluted from gels following D-R of an intergenic isozyme showed that the Adh ₂ isozymes were more than twice as active as those of Adh ₁. Measurements of activities of crude extracts from the four possible double homozygous genotypes indicated that the seeds of the genotype Adh ₁ ^F /Adh ₁ ^F , Adh ₂ ^S /Adh ₂ ^S produced more activity than the other three. This genotype is the most common one found in wild and cultivated stocks. Isozymes eluted following electrophoresis of the same extracts had averages of 19%, 70%, and 11% of total activity contributed by the Adh ₁, Adh₂, and intergenic isozymes, respectively. A simple but efficient method of isozyme elution from starch gels is described which resulted in nearly full expected recovery (approximately 46%) of the ADH activity in the applied sample.Supported by Graduate School and BioMed grants and by NSF Grant GB35853.     

Isozyme variation in Verticillium dahliae isolates from Crete

Fifteen isolates ofVerticillium dahliae (eight of race1, seven of race2; most from the island of Crete, Greece) were examined for isozyme and molecular variation. Among the isozyme banding patterns (zymograms) of six enzymes that were “activity-stained” after electrophoresis in 9% polyacrylamide gels, differences were observed in diaphorase, α-esterase, peroxidase and superoxide dismutase; 2, 2, 3 and 5 different types of zymograms were recorded, respectively. The zymograms could not be correlated with either race1 or2. However, all six isolates originating from the Oropedio (plateau) are, of Lasithi (Crete) showed an esterase zymogram clearly distinguishable from the other isolates. No differences were observed when staining for acid phosphatase or aspartate aminotransferase (‘glutamic-oxaloacetic transaminase’). Furthermore, electrophoresis of random-amplified polymorphic DNA (RAPD) in 2% agarose gels showed that three race-2 isolates from Oropedio of Lasithi could also be distinguished by the RAPD pattern generated with primer OPA-1. The variation observed possibly represents adaptation ofV. dahliae to the Oropedio environment.     

Cross-amplification of microsatellites from the codling moth Cydia pomonella to three other species of the tribe Grapholitini (Lepidoptera: Tortricidae)

This study examined cross-species amplification of 33 microsatellite markers, previously developed for Cydia pomonella, in three related fruit moth species of the same tribe (Grapholitini), namely Grapholita molesta, Grapholita funebrana and Grapholita lobarzewskii. Eight microsatellite loci yielded polymorphic products for G. molesta, nine for G. funebrana and 11 for G. lobarzewskii. At all these loci, the number of alleles ranged between four and 11 in G. molesta, and between four and nine in G. funebrana and G. lobarzewskii each. The successful cross-amplified loci can be used for research on population genetics and gene flow of the three target species.     

Isozyme patterns in callus cultures and in plants regenerated from calli ofCereus peruvianus (Cactaceae)

Electrophoretic patterns for isocitrate dehydrogenase (IDH; EC 1.1.1.42), acid phosphatase (ACP; EC 3.1.3.2), peroxidase (PER; EC 1.11.1.7), and esterase (EST; EC 3.1.1.1) isozymes were determined inCereus peruvianus tissues and used as markers of genetic uniformity of calli and of the plants regenerated from callus cultures. One IDH, six ACP, six PER, and six EST isozymes were induced in cultured callus tissues in medium containing three 2,4-dichlorophenoxyacetic acid and kinetin combinations. Four ACP, two PER, and three EST isozymes were still present in all regenerated plantsin vitro and therefore can be used as markers of theC. peruvianus plants regenerated from callus tissues. The differential patterns of ACP and IDH isozymes and the similar zymograms for PER and EST isozymes presented by callus tissues were used in a comparison of callus tissues cultured for 2 years. The comparative analysis of zymograms within each enzyme system indicated a mean heterogeneity coefficient of 0.33 forC. peruvianus calli cultured for 2 years. Because of the isozyme variations, which developed in culture medium and were transferred to the regenerated plants, the IDH, ACP, PER, and EST enzyme systems can be considered to be good markers for investigating possible genetic variations in plant populations ofC. peruvianus obtainedin vitro from callus culture.This research was supported by the CNPq     

Allozyme variation in stable flies (Diptera: Muscidae)

Polyacrylamide gel electrophoresis was used to resolve allozymes in the cosmopolitan blood-feeding stable fly,Stomoxys calcitrans (L.). Nineteen of 38 loci were polymorphic (53%). Mean heterozygosities among all loci and among only polymorphic loci were 0.096 and 0.182, respectively. These gene diversity measures are about half those among other muscid Diptera. Variation in gene frequencies was examined in 10 natural stable fly populations from Iowa and Minnesota. Gene frequencies were homogeneous at five of eight loci among six populations in 1990 and eight of eight loci among four populations in 1992. Wright'sF statistics showed no significant departure from random mating among stable flies. It was concluded that gene flow compensates for any local differentiation in stable fly populations.