携带人野生型PKGⅠα基因的重组腺病毒载体的构建及鉴定

目的:克隆人PKGⅠa基因,构建其重组腺病毒载体。方法:用RT-PCR方法从人肺动脉平滑肌组织中扩增PKGⅠa基因全长,经T/A克隆后,亚克隆至腺病毒穿梭质粒pAdTrack-CMV上,构建穿梭质粒pAdTrack-PKGⅠα。PmeⅠ酶切pAdTrack-PKGⅠα,然后分别将腺病毒骨架质粒pAdEasy-1和穿梭质粒pAdTrack-PKGⅠα转化至BJ5183感受态细菌中进行同源重组,PacⅠ酶切线性化重组质粒AdCMV-PKGⅠα后转染Ad293细胞进行病毒包装和扩增。检测PKGⅠα基因的表达,并用绿色荧光蛋白(GFP)法测定其滴度。结果:用RT-PCR方法,从人肺动脉中层扩增出PKGⅠα,测序证实为人PKGⅠα基因。构建了PKGⅠα基因的重组腺病毒载体并制备出高滴度重组病毒保存液。结论:成功地克隆了人PKGⅠα基因,并构建其重组腺病毒载体,为进一步研究PKGⅠα基因在低氧肺血管重建中的作用提供了有效的基因转移载体。

Phylogeny of Apaturinae Butterflies (Lepidoptera: Nymphalidae) Based on Mitochondrial Cytochrome OxidaseⅠ Gene

The phylogenetic relationships of genera in the subfamily Apaturinae were examined using mtDNA sequence data from 1,471 bp of cytochrome oxidase subunit Ⅰ （COI）. The mitochondrial COI gene from a total of 16 species in 11 genera were sequenced to obtain mtDNA data, along with those of 4 species obtained from GenBank, to construct the MP and the NJ trees using Athyma jina, Penthema adelma, Polyura nepenthes, and Charaxes bernardus as outgroups. The transitions at the third codon positions of the COI data set were found saturated, but they were retained for analysis, because they contain the majority of the phylogenetic information. The impacts of equal weight assumptions for all characters in the parsimonious analysis were assessed by potential alternations in clades in response to different transition/transversion weighting schemes. The results indicated four distinct major groups in Apaturinae. Moreover, several well supported and stable clades were found in the Apaturinae. The study also identified undetermined taxon groups whose positions were weakly supported and were subject to changes under different weighting schemes. Within the Apaturinae, the clustering results are approximately identical to the classical morphological classification. The mtDNA data suggest the genus Mimathyma as a monophyletic group. Lelecella limenitoides and Dilipa fenestra have close relationship with very strong support in all phylogenetic trees. It also supports the taxonomic revision of removing several species from Apatura to other genera, namely Mimathyma schrenckii, M. chevana, M. nycteis, Chitoria subcaerulea, C. fasciola, C. pallas, and Helcyra subalba.

Development and Clinical Application of a Single-tube Nested PCR Method to Amplify the DNA Polymerase Ⅰ Gene of Treponema Pallidum

Objective: To develop a sensitive, specific and simple method for detection of extremely low numbers of T. pallidum in clinical specimens, as a significant addition to the serologic tests for syphilis diagnosis. Methods: Double-tube nested PCR(DN-PCR) and single-tube nested PCR(SN-PCR) assays were performed to amplify specific fragments of the DNA poly-merase I gene(polA) of T. pallidum. Sensitivity and specificity of the two PCR assays were tested. Eighty-six whole blood specimens from persons with suspected syphilis were detected by the two nested PCR methods. The TPPA test was used as a comparison for detecting syphilis in sera from corresponding patients. Results: Only specific amplicons could be obtained during amplification of the T. pallidum polA gene and the detection limit was approximately 1 organism when analyzed on gel by the two PCR methods. Of 86 clinical specimens, 62 were positive by TPPA. Of these, 54 and 51 were positive by the DN-PCR and SN-PCR, respectively, which does not represent a statistically significant difference between the two PCR tests. Of 24 TPPA-negative specimens, 5 were positive by both DN-PCR assay and SN-PCR assay. Conclusion: The SN- polA PCR method is extremely sensitive, specific and easy to perform for detecting low numbers of T. pallidum in clinical blood specimens as a complementary to serology for syphilis diagnosis.

小鼠前扣带回皮质PKG-Ⅰ介导吗啡诱导的痛敏和焦虑样行为

目的:探讨前扣带回皮质cGMP依赖的蛋白激酶-Ⅰ(PKG-Ⅰ)在吗啡诱致的小鼠痛敏及焦虑样行为中的调控作用。方法:将雄性C57BL/6小鼠随机分为2组:对照组和吗啡组,在小鼠皮下每天两次、连续4 d注射吗啡建立吗啡诱致的痛敏模型。分别采用von Frey纤维丝和高架十字迷宫检测小鼠机械性痛阈变化和焦虑样行为。通过Western Blot和免疫荧光组织化学染色技术检测前扣带回皮质PKG-Ⅰ表达水平的变化。结果:长期大量皮下注射吗啡可诱致小鼠产生显著的痛觉敏化和焦虑样行为。Western Blot结果显示小鼠前扣带回皮质PKG-Ⅰ在吗啡诱致的痛敏后表达显著下调,同时免疫荧光组织化学染色结果显示前扣带回皮质PKG-Ⅰ在吗啡痛敏后的平均荧光强度显著下降。结论:前扣带回皮质PKG-Ⅰ在吗啡诱致的小鼠痛觉过敏和焦虑样行为中发挥关键作用。

Analysis of Rb gene Xba Ⅰ polymorphism in Shaanxi aged atherosclerosis population

Objective:To investigate variable number tandem repeat (VNTR) polymorphism of the 17th intron of Rb gene in Shaanxi aged population and the relationship between the polymorphism of Rb gene and atherosclerosis(AS) genetic suscepti- bility. Methods: VNTR polymorphism of the 17th intron of Rb gene were examined in 100 Shaanxi aged AS patients and 100 Shaanxi aged control individuals by PCR-Rb-Xba Ⅰ-RFLP. Results::Two alleles were found both in AS group and control group, which were separately 945 bp(S1) and 630bp + 315bp(S2). S1S2 genotype was the most frequent one in the two populations. Significant difference in allele frequency was not found between AS group and control group, and allele frequency was no significant difference between Chinese and Caucasian. Conclusion: Xba Ⅰ enzyme site of Rb gene could have been certainly stable in AS population, and it was inferred that the polymorphism locus was not liable to cause mutation, which might not implicated in the formation of AS.

The gene diagnosis and mutation survey of autosomal dominant polycystic kidney disease Ⅰ

Objective: To explore gene diagnosis of autosomal dominant polycystic kidney disease (ADPKD Ⅰ ),and to look for the typical mutation in order to improve the gene diagnosis. Metbods: southern blot and PCR wasused to observe the mutation condition of 3' end single copy region of ADPKD Ⅰ gene ; Amplifying and analyzingthe microsatellite SM7 by PCR. Results: ①After the probe AH4 was hybridized with 16 patients' genomic DNAby Southern blot, the common 15 kb fragments were found in every one; ②For 27 patients, 5. 72 kb genomicDNA, which is between the probe AH4 and JH14, was amplified by PCR, and no 5. 5 kb genomic DNA deletionwas found in this region; SM7 was amplified in lO9 health persons, its PIC was 0.76, and was closely linked towith ADPKD Ⅰ gene in three patient families. Conclusion: In Han nation, ①No large genomic DNA segmentdeletion could be found frequently in ADPKD Ⅰ gene 3' end single copy region; ②The PIC of SM7 is high, it canbe used to make rapid gene diagnosis in about 70% ~80% ADPKD Ⅰ families.

Establishment of a Real-time Fluorescent Quantitative RTPCR Method for Detecting NP Gene of Class Ⅰ Newcastle Disease Virus(NDV)

Newcastle disease( ND) is one of the most serious infectious diseases that infect the poultry industry.There is only one serotype of Newcastle disease virus( NDV),but NDVs can be divided into two distinct classes( class Ⅰ,and class Ⅱ) according to their genetic relationship.To develop a method for rapid quantitative detection of class Ⅰ NDV,a pair of primers and a TaqM an probe were designed and synthesized according to the conservative sequence of NP gene of class Ⅰ NDV.The positive recombinant plasmid harboring NP gene of JS-18-05 isolate was used as a positive template to establish the standard curve.A real-time fluorescent quantitative RT-PCR method was established for rapid detection of class Ⅰ NDV with strong specificity,high sensitivity and good repeatability.The established method exhibited a good linear relationship within the concentration of 102 to 108 copies of NDV,by which 1 μl of 10 copy of NDV nucleic acid could be detected in the initial template.Compared with conventional virus isolation methods,the established method had similar sensitivity and led to the same results in detecting33 class Ⅰ,class Ⅱ NDV isolates.The study provided the basis for rapid quantitative detection of class Ⅰ NDVs and further clarification of their pathogenicity and pathogenic mechanism in poultry.

Inhibition of α_1(Ⅰ) collagen gene in vitro transcription by antisense oligodeoxynucleotides

Objective and Methods: Excessive accumulation of collagen typeⅠ and type Ⅲ causes the formation of keloids and hypertrophic scars. To understand the mechanism by which antisense oligodeoxynucleotide (Oligo) acts on in vitro transcrption α1 (I) collagen gene, isotopes (α-32pGTP) was incorporated into 2 SP6 in vitro transcription systems. Results and Conclu- sion: Oligo 2 (at the transcription start region) could effectively inhibit in vitro transcription of pGEM3-Col13 and the control (random oligodeoxynucleotides) showed no inhibition. However, oligo 1 (at the transcription start region) obviously inhibited the in vitro transcription of pGEM3-Col14, while Oligo 2, which targeted at the down stream region (about 200 bp) of the promoter showed no significant inhibition effect.

南疆部分地区绵羊捻转血矛线虫苯并咪唑抗性相关分子Ⅰ型β-微管蛋白基因的多态性分析

为了解南疆地区绵羊捻转血矛线虫对苯并咪唑类药物的抗性相关分子β-微管蛋白基因的多态性,本研究对克州及喀什的183条捻转血矛线虫成虫进行ITS-2基因特异性PCR鉴定后,对抗药相关的Ⅰ型β-微管蛋白基因进行了扩增和测序,并对该抗药基因的单核苷酸多态性(SNP)167、198和200位点进行了分析。结果:在2个地区种群中,198位点及200位点均发生不同程度突变,且以198位点突变为主,暂未在167位点发生突变;两地共发现了5种基因型,其中198位点纯合敏感型及200位点纯合抗药型(喀什12条占12.37%,克州2条占2.33%),198位点纯合抗药型及200位点纯合敏感型(喀什23条占23.71%,克州7条占8.14%)两地均存在,提示这2个种群都存在抗药性。本研究首次报道了南疆部分地区捻转血矛线虫种群Ⅰ型β-微管蛋白基因存在苯并咪唑类药物抗药性突变,为新疆地区捻转血矛线虫病的有效防控及抗药性研究提供理论依据。

The Genetic Structure and Diversity of Repomucenus curvicornis Inhabiting Liaoning Coast Based on Mitochondrial COⅠ Gene and Control Region

[Object] This study was conducted to explore the genetic diversity and structure of the wild Repomucenus curvicornis inhabiting Liaoning Coast, China. [Method] The mitochondrial COⅠ gene and control region（CR） were PCR amplified from the wild R. curvicornis populations from the Liaodong Bay（n=22） and the northern Yellow Sea（n=18）, sequenced and analyzed for genetic diversity. [Result] The contents of A, T, C and G of 624 bp COⅠ gene were 24.09%, 31.04%, 25.28%, and 19.59%, and those of 460 bp CR fragment were 32.96%, 32.80%, 14.86% and 19.38%, respectively. The total number of variable sites, average number of nucleotide differences（ k）, haplotype diversity（H） and nucleotide diversity（π） based on COⅠ gene were 38, 4.67,（0.96±0.02） and（0.007 5±0.004 2）, and those based on CR fragment were 26, 3.35,（0.97 ±0.02） and（0.007 3±0.004 3）, respectively. Based on mitochondrial COⅠ gene and CR, the genetic diversity of Liaodong Bay population was lower than that of the northern Yellow Sea population. The AMOVA analysis based on CR fragments revealed almost significant genetic divergence between the Liaodong Bay and the northern Yellow Sea populations, while there was no significant genetic divergence based on COⅠ gene. The results showed that CR and COⅠ gene are effective molecular markers for detecting the genetic diversity of R. curvicornis population, while CR is more reliable than COⅠ gene in detecting the genetic structure. [Conclusion] CR is an appropriate marker for genetic analysis of marine fish population.

The Truncated Gene cfaD′ Positively Regulates CFA/Ⅰ Expression of Enterotoxigenic Escherichia coli

The gene cluster cfaABCED’ of enterotoxigenic Escherichia coli, encoding the fimbriae which is called colonization factor antigen located on a plasmid. It is positively regulated by cfaR, a member of the AraC family, and the cfaD’ gene region, which is located downstream of cfaE and is homologous to cfaR, had been described as a truncated cryptic gene. In the present study we observed that the CFA/ fimbriae subunit, cfaB, was expressed in lower amount by the cfaABCED’ clone pNTP513 in host E. coli HB101. The expression of CFA/ diminished by deletion of cfaD’ gene region from pNTP513, and was restored by acquisition of cfaD’ in trans. Furthermore, CFA/ expression by cfaD’ deletion mutant, the cfaABCE clone, was remarkably increased by the presence of cfaD’ in trans in a topoisomerase A deficient strain of E. coli DM800. These data suggest that cfaD’ region is a functional region of gene, that regulates the CFA/ expression with cfaR by unknown mechanism.

雀形目15种鸟类CoⅠ与Cyt b基因序列的比较

对雀形目Passeriformes6科15种鸟类线粒体DNA的Cyt b基因全序列(1143bp)和CoⅠ基因部分序列(1176bp)进行了比较,结果显示Cyt b和CoⅠ基因序列的变异位点分别为454个和366个,简约信息位点为337个和303个,而且CoⅠ基因比Cytb基因略微保守,进化速率也较低。采用邻接法、最大简约法、最大似然法和贝叶斯法分别构建了CoⅠ和Cyt b基因两组数据集的分子系统发生树及其合一树,并对建树结果进行了比较分析。基于以上两点,本文认为CoⅠ基因比Cyt b基因更适合于确定雀形目科级阶元之间的系统发生关系,而且它也能够作为雀形目物种鉴定的分子标记,但在物种鉴定方面不如Cyt b基因稳定和准确。

湖羊GHR和IGF-Ⅰ基因表达的发育性变化及其与肉质性状的关联

【目的】探讨生长激素受体(growth hormone receptor,GHR)和胰岛素样生长因子-Ⅰ(insulin-likegrowth factor-Ⅰ,IGF-Ⅰ)基因在湖羊不同生长阶段背最长肌中表达丰度与肉质性能的相关性以及这两个基因表达水平的关联性,为湖羊肌肉生长性状的选育提供遗传学资料。【方法】利用荧光定量RT-PCR分析GHR和IGF-Ⅰ基因在湖羊早期生长背最长肌肉组织中的mRNA的发育性变化。【结果】①出生后随着月龄的增加,母羊GHR基因在背最长肌的表达趋势为:先升高后降低再升高再降低最后再升高,最后6月龄到达最高点;公羊GHR在背最长肌的表达趋势为:先升高到2月龄到达一个峰值,2月龄到4月龄为一个降低的过程,4月龄到6月龄又升高,并到达最高点;母羊IGF-Ⅰ基因在背最长肌的表达趋势为:由2日龄开始依次升高最后于6月龄到达最高点;公羊IGF-Ⅰ基因在背最长肌的表达趋势为:先升高到1月龄到达一个峰值,1月龄到3月龄为一个降低的过程,并于3月龄降至与初生接近相等的水平,此后随月龄增加逐渐升高,并于6月龄到达最高点;②GHR和IGF-Ⅰ基因在湖羊各月龄间大多存在显著或极显著差异,湖羊的公羊和母羊的GHR和IGF-Ⅰ基因的相同生长阶段的表达也大多存在显著或极显著差异;③GHR和IGF-Ⅰ基因的表达存在显著正相关(0.01<P<0.05),GHRI和GF-I基因与肌纤维直径均存在极显著正相关(P<0.01),GHR与肌纤剪切力存在极显著正相关(P<0.01),IGF-Ⅰ与肌纤剪切力存在显著正相关(0.01<P<0.05),GHR和IGF-Ⅰ基因与肌纤维密度均存在极显著负相关(P<0.01)。【结论】性别和年龄对于GHR和IGF-Ⅰ基因在湖羊不同生长阶段的肌肉中的表达具有重要影响;出生后,各基因表达水平并非随之上升或者下降,各基因表达水平出现拐点的时间并不相同;GHR和IGF-Ⅰ基因在湖羊早期肌肉性状的表达为显著正相关,可以作为湖羊早期肉质性状的候选基因。

人胰岛素样生长因子Ⅰ在大肠杆菌中的表达研究

胰岛素样生长因子Ⅰ（ＩＧＦ－Ⅰ）是一种多功能细胞增殖调控因子，它对许多疾病有较好的治疗作用．为了获得大量的ＩＧＦ－Ⅰ产品，在测定了ＩＧＦ－Ⅰ全长序列的基础上，构建了ＩＧＦ－Ⅰ表达载体ｐＢＶＩＧＦ，经热诱导表达后，ＳＤＳ－ＰＡＧＥ分析表明：含有重组表达质粒的菌株可表达出７．６ｋＤ的蛋白．研究了不同菌株对ＩＧＦ－Ⅰ表达的影响．ＩＧＦ－Ⅰ的表达水平可达１５ｍｇ／Ｌ．重组蛋白主要以包涵体形式存在，进行了初步纯化和复性研究，Ｗｅｓｔｅｒｎ印迹表明重组蛋白具有ＩＧＦ－Ⅰ的抗原性．并初步建立了ＩＧＦ－Ⅰ生物活性测定方法．

PCR-RFLP技术对Ⅰ群禽腺病毒12个血清型毒株的分型鉴定

应用扩增Ⅰ群禽腺病毒(AAV)Hexon基因A片段和B片段的2对引物,对Ⅰ群AAV的12个血清型毒株进行了PCR扩增。结果扩增出的A片段大小为1 219 bp,B片段大小为1 350 bp。对A片段用限制性内切酶HaeⅡ进行酶切,结果得到6种不同的RFLP图谱;对B片段进行HaeⅡ酶切,结果得到9种不同的RFLP图谱。综合分析A片段和B片段的PCR-RFLP结果,能鉴别Ⅰ群AAV的12个血清型。结果表明,建立的PCR-RFLP具有快速、简单、特异、灵敏等优点,可作为Ⅰ群AAV流行毒株血清型的快速分型工具。

基于cox Ⅰ基因对猪囊尾蚴河南分离株种系发育关系的研究

利用RT-PCR技术从河南部分地域的猪囊尾蚴中获得10个分离株的cox Ι部分基因序列,其长度为344bp;将其克隆入pMD19-T并测序;分别用Clustal X 1.81程序对序列进行比对,然后用PAUP 4.0程序MP法和NJ法绘制种系发育树,并用PUZZLE 5.2程序构建最大似然树;同时利用WDANSIST 2.5程序和DNAstar 5.0中的Megalign程序进行同源性分析。结果表明,10个河南猪囊尾蚴分离株的coxΙ部分基因序列完全一致,属于猪带绦虫亚洲基因型;猪囊尾蚴coxΙ部分基因可有效区分出Asian和American/African两种基因型,并可用于不同种带科绦虫的鉴别诊断。因此,猪囊尾蚴coxΙ基因有望作为一种鉴别基因用于带科绦虫病和囊尾蚴病的PCR鉴别诊断。

我国汉族人群HLAⅠ类经典基因单倍型及连锁分析

本研究旨在探讨我国汉族人群HLAⅠ类经典基因座位HLA-A、HLA-B、HLA-Cw位点的基因频率,单倍型频率及连锁特征。采用序列特异性引物(SSP)PCR低分辨基因分型技术对1014例随机选择的无关个体的经典HLAⅠ类位点进行基因分型,并对其相关遗传学参数进行统计学分析。结果发现汉族人群中较为常见的HLA-Ⅰ类基因是A*02(0.33)、A*11(0.24)、B*15(0.14)、B*13(0.13)、Cw*03(0.25)、Cw*07(0.18);较为常见的单倍型是A*02-B*46(0.071)、A*11-B*15(0.051)、A*02-Cw*01(0.084)、A*11-Cw*03(0.079)、B*46-Cw*01(0.095)和B*13-Cw*03(0.071)等,其中A*02-B*46、A*30-B*13、A*30-Cw*06、A*02-Cw*01、B*46-Cw*01和B*58-Cw*03等单倍型呈现出显著的连锁不平衡;而A*02-B*15、A*02-B*40、A*24-Cw*03、A*02-Cw*03、A*31-Cw*03等连锁不平衡性相对较低,其中A*24-Cw*03在重组事件中较常出现。此外,A*02-B*46-Cw*01(0.075)、A*30-B*13-Cw*06(0.046)、A*11-B*13-Cw*03(0.045)、A*33-B*58-Cw*03(0.044)、A*11-B*15-Cw*08(0.027)、A*02-B*38-Cw*07(0.023)、A*11-B*40-Cw*07(0.022)等为常见扩展单倍型。结论:本研究较系统地分析了我国汉族人群的HLA遗传学分布特点,为群体进化、临床移植及疾病相关研究等提供了有价值的遗传学资料。

中华虎头蟹线粒体16S rRNA和 COⅠ基因的序列比较及其系统进化分析

为研究中华虎头蟹野生群体的种质资源及遗传多样性状况,采用PCR扩增获得中华虎头蟹线粒体DNA的16S rRNA和COⅠ基因片段,分别对其进行序列比较及系统进化分析。16S rRNA和COⅠ基因片段的A+T平均含量分别为67.7%和61.4%,A+T含量显著高于G+C含量。长度为515 bp的16S rRNA基因片段共检测出单倍型4种,多态性位点4个,均为单一变异位点;长度为653 bp的COⅠ基因片段共检测出单倍型11种,多态性位点23个,其中简约信息位点5个和单一变异位点18个。COⅠ基因片段比16S rRNA基因片段具有较大的变异,更适于中华虎头蟹种群的遗传多样性分析。基于16S rRNA和COⅠ基因片段的遗传距离与系统进化分析结果一致,表明中华虎头蟹与梭子蟹科的蟹类亲缘关系最近,方蟹科与沙蟹科的蟹类聚为一支,与传统分类结果基本一致;而脊椎动物2个基因片段的系统进化分析结果不一致。根据16S rRNA基因片段的遗传距离推测出4科7种蟹的大致分化时间发生在古新世至始新世。

罗氏沼虾3个群体线粒体COⅠ基因的序列差异和遗传标记研究

利用PCR方法扩增获得罗氏沼虾(Macrobrachium rosenbergii)线粒体DNA的COⅠ基因,测定该基因片段序列。分析了罗氏沼虾缅甸原种F1代、江苏养殖群体和广西选育F2代3个群体共17只个体的序列核苷酸位点差异和遗传多态。结果表明,缅甸原种F1代遗传多样性最为丰富,江苏养殖群体和广西选育群体的遗传多样性相对贫乏。在长度为498 bp的基因片段中,共检测到10个多态性核苷酸位点(占2.01%),17只个体具有5种基因型,3群体各自的平均核苷酸位点差异分别为0.88%、0.07%和0。UPGMA分子系统聚类树显示,江苏养殖群体和广西选育群体的遗传关系最近,其单倍型混杂聚成一支,而缅甸原种F1群体相对独立为另外一支。COⅠ基因可以作为区分两分支群体的遗传标记。

鸡IGF-Ⅰ基因SNPs及其对屠体性状的遗传效应分析

以180只3个品系的温岭草鸡为材料,采用PCR-RFLP方法测定了IGF-Ⅰ基因的3个SNPs座位,同时分析了它们对屠体性状的遗传效应。结果显示:PstⅠ、HinfⅠ和TaqⅠ识别座位分别发生T→C、C→A和C→T突变,每个SNPs座位各出现了3种基因型,其中A系在3个座位上均处于Hardy-Weinberg平衡状态(Ρ>0.05)。方差分析显示每个座位基因型对部分屠体性状都有极显著或显著的差异(Ρ≤0.01或0.01<Ρ≤0.05)。多重比较显示:在其中6个屠体性状上,每个座位3种基因型的最小二乘均值之间均有突变型>杂合型>野生型的关系,联合基因型QF/QF和QE/QF的最小二乘均值在4个屠体性状上显著高于(0.01<Ρ≤0.05)联合基因型PE/QE,每个座位突变等位基因都对部分屠体性状具有增效作用。A系和B系之间的遗传距离为0.005 3,聚类分析表明两系同为1枝。