尘螨变应原Der fl全序列的原核表达及生物信息学分析

目的 构建尘螨变应原Der fl原核表达体系,并了解其分子特征。方法 提取粉尘螨总RNA,用RT—PCR合成Der fl编码基因,将其克隆至pMD19-T载体,亚克隆至表达载体pET-28a（＋）,转化至大肠杆菌并刚IPTG诱导表达。用生物信息学软件对测序结果进行分析并预测其空间结构。结果从粉尘螨总RNA中扩增获得Der fl cDNA片段,成功构建了表达质粒pET-28a（＋）-Der fl,Western blotting显示原核表达获得成功。测序结果提交GenBank,臀陆号为EU095368,该基因长966bp,与参考序列同源性达99．9％,推测其编码氩基酸321个,属疏水蛋白,位于细胞外,信号肽位于1～18氨基酸处。同源性分析提示Der fl和Eur ml相似率为88％,而Der fl和Derpl的相似率为77％,分子进化树中粉尘螨和梅氏嗜霉螨聚成一簇。Derfl的二级结构由α-螺旋（109aa,33．96％）、延伸链（55aa,17．13％）、β-转角（18aa,5．61％）和随机卷曲（139aa,43．30％）组成：结论 尘螨变麻原Der fl原核表达获得成功,为进一步生产重组变麻原奠定了基础。生物信息学分析表明粉尘螨和梅氏嗜霉螨的亲缘关系可能更近,而与屋尘螨关系稍远,此与现行的形态学分类系统并不符合。     

美洲大蠊变应原Per a 2的生物信息学分析

目的：了解美洲大蠊变应原Per a 2的分子生物学特征。方法：从Genbank中获得Per a 2的核酸序列,用ExPaSy、EBI和NCBI网站的在线软件推导出编码氨基酸序列及其理化性质、空间结构、功能位点,并在Blastp比对后选择不同物种同源序列计算井刖双率、构建分子进化树。结果：Per a 2由351个氨基酸细戍,分子量为38119Da、等电点为490、分子式为C1217H1825N285O297S18,为细胞外疏水性蛋白、属于肽酶a家族,信号肽位于1～20氨基酸处,三个跨膜螺旋区域依次位于1～19aa、51～78aa、282～300aa处;二级结构由α-螺旋（9．4％）、β延伸（28．49％）、随机线圈（62．11％）组成;美洲大蠊和德国小蠊相似率为55％、与马德拉蜚蠊相似率为51％,三者在Per a 2与不同物种的同源序列构建的分子进化树中聚成一簇。结论：通过对Per a 2的生物信息学分析获得了该变应原分子特征．为进一步研究奠定基础。     

粉尘螨线粒体样苹果酸脱氢酶基因cDNA克隆和分子特征分析

摘要 目的：获取粉尘螨线粒体样苹果酸脱氢酶蛋白（mitochondrial-like malate dehydrogenase，mMDH）的编码基因并了解其分子特征。方法：以粉尘螨Total RNA为模板，RT-PCR扩增获得mMDH编码基因后、构建原核表达质粒，转化E.coil BL21(DE3)感受态细胞中，IPTG诱导表达，SDS-PAGE和Western Blot鉴定目的蛋白表达情况。采用NCBI、EXPASY在线生物信息学软件分析该基因编码蛋白质的生物学特征。结果：获得粉尘螨线粒体样苹果酸脱氢酶蛋白的编码基因，全长1032bp。构建的原核表达质粒pET28a(+)-mMDH，经转化和诱导表达后，SDS-PAGE和Western Blot可见目的蛋白条带。该基因编码的蛋白质由343个氨基酸组成，相对分子质量（Mr）36014.54Da，亚细胞定位主要在细胞质和细胞核，含有34个磷酸化位点（19个丝氨酸，12个苏氨酸和3个酪氨酸）。糖基化预测结果显示其含有2个N-糖基化位点（123位存在糖基化位点NASI和151位存在糖基化位点NSTV）和1个0-糖基化位点。二级结构主要为?琢-螺旋和无规则卷曲。三维建模可观察到该蛋白为二聚体结构，CD-Search保守区域分析后显示其属于NADB-Rossmann家族，具有MDH-glyoxysomal-mitochondrial结构域。PyMol可视化后可在三维结构中观察到保守区域位点。将该基因推导出的氨基酸序列进行Blast获得同源基因，粉尘螨与屋尘螨、梅氏嗜霉螨进化关系较近，独成一簇。结论：获得粉尘螨线粒体样苹果酸脱氢酶蛋白的编码基因全长及其原核表达质粒，并对其生物学特征进行分析，为进一步探讨该基因的生理功能、开发尘螨控制措施奠定基础。     

四份中国HCV阳性血清中包膜蛋白E1/E2准种基因的序列分析及新型插入突变的发现

为分析四份中国丙型肝炎病毒（HCV）阳性血清中包膜蛋白E1/E2基因的准种特征。本研究对从4份中国HCV阳性血清（1b亚型：274、366、383;2a亚型：283）中提取的HCV核酸,采用逆转录-聚合酶反应扩增编码全长E1/E2蛋白（191～764aa）的基因片段,随机挑取多个克隆测序。根据E1/E2基因核苷酸的序列与其他相关序列（来自于GenBank）构建亲缘性关系进化树,进行核苷酸与氨基酸同源性分析并对重要的基因位点进行分析。共获得阳性克隆序列43个（274株10个,283株12个,366株13个,383株8个）,发现高变区HVR1、HVR2的基因异质性高,而其他抗体中和表位及跨膜区I、II及N末端糖基化位点相对保守。并首次发现在HCV 2a亚型（283血清）中多个准种序列存在1279nt（E1区,313aa）处单碱基插入优势基因突变,导致HCV包膜蛋白编码突变与中断（E2区,398aa）。本研究对中国HCV代表株包膜蛋白E1/E2编码基因的准种多样性及一种新型插入突变进行了描述,可为进一步研究HCV免疫逃避与慢性化机制提供重要信息。关键词：丙型肝炎病毒;包膜蛋白;序列分析;准种;插入突变     

鸽源H5N1亚型禽流感病毒株的HA和NA基因特征性分析

本研究自行设计合成两对特异性引物,通过RT-PCR扩增出1株鸽源H5N1亚型禽流感病毒血凝素（HA）和神经氨酸酶（NA）两个基因的cDNA片段,将它们成功克隆于pMD18-T载体上,然后进行序列测定。结果表明,HA基因全长1707bp,编码568个氨基酸, HA基因有7个糖基化位点,在裂解位点附近有连续6个碱性氨基酸（R-R-R-K-K-R）的插入,具有高致病性毒株的分子特征。受体结合位点的氨基酸分别为YWIHELY,左侧壁氨基酸为SGVSSA,右侧壁为NGQSGR;NA基因全长1350bp,编码446个氨基酸,NA基因有3个糖基化位点。     

冰核细菌(Erwinia ananas 110)冰核基因克隆和序列分析

从作者自行分离的冰核细菌（Erwinia ananas110)中克隆到我国第1个细菌冰核基因,并完成其序列测定和分析,所克隆基因编码区全长3921bp,编码1306aa,氨基酸序列明显分为3个区即N-端（161aa),C-端（41aa)的单一序列区和中部的高度重复序列R区（1104aa)。以16氨基酸为重复单元的R区占整个编码序列的84.5%。序列分析表明我们所克隆的基因为一个新冰核基因,将其命名为iceA。该基因已在GenBank上登录,登录号为：AF387802。     

红树植物秋茄中受盐胁迫抑制的cyclophilin基因的鉴定与表达分析

利用代表性差异分析方法获得秋茄中两个编码亲环素(cyclophilin)蛋白的cDNA片段(称为SRGKC2和SRGKC3),该片段大小分别为282bp和160bp;序列分析表明：SRGKC2和SRGKC3是同一基因区域的不同长度片段,SRGKC3是SRGKC2片段的一部分。SRGKC2在84个氨基酸范围内与大戟属cyclophilin蛋白的氨基酸序列的一致性达到90％,SRGKC3在47个氨基酸范围内与蚕豆cyclophilin蛋白的一致性达到93％。Northern分析表明：盐分抑制SRGKC2片段的表达。依赖SRGKC2片段的序列资料,利用cDNA快速末端扩增(RACE)技术获取秋茄中cyclophilin基因的全长cDNA片段(命名为KCCYP1)(GenBank登录号：AY150052)。该cDNA全长约为0．9kb,含有一个516个核苷酸的完整开放阅读框,编码172个氨基酸,等电点为8．57,分子量18．2KDa。42—49位氨基酸残基为推测的ATP／GTP结合位点A基序(P—loop),48—54位氨基酸残基是插入的7个氨基酸残基。文中还对SRGKC2在不同种中的表达状况进行了分析。     

粘虫核糖体蛋白S7cDNA的克隆和表达分析

运用RT—PCR和RACE技术克隆了粘虫Mythimnaseparata（Walker）核糖体蛋白s7基因（RPS7）的全长eDNA序列（GenBank登录号：JN582331）,并对其进行生物信息学分析。结果表明,粘虫RPS7全长eDNA序列为762bp,包括5’非编码区32bp和3’非编码区67bp。其开放阅读框（573bp）编码190氨基酸肽链,具有核糖蛋白S7e蛋白家族典型特征。该肽链理论分子量为21．924ku,等电点为9．82,富含4种类型的特定功能位点。该蛋白序列与其他动物RPS蛋白序列具有96．8％-98．2％高度同源性。应用荧光实时定量技术建立了粘虫脑部胚后发育RPS7表达模式。RPS7表达量随胚后发育脑部重建呈现出动态变化,这一结果显示RPS7是在转录水平上呈现发育性调节。     

尘螨变应原Der f1全序列的原核表达及生物信息学分析

目的 构建尘螨变应原Der f1原核表达体系,并了解其分子特征.方法 提取粉尘螨总RNA,用RT-PCR合成Der f1编码基因,将其克隆至pMD19-T载体,亚克隆至表达载体pET-28a( ),转化至大肠杆菌并用IPTG诱导表达.用生物信息学软件对测序结果进行分析并预测其空间结构.结果 从粉尘螨总RNA中扩增获得Der f1 cDNA片段,成功构建了表达质粒pET-28a( )-Der f1,Western blotting显示原核表达获得成功.测序结果提交GenBank,登陆号为EU095368,该基因长966 bp,与参考序列同源性达99.9%,推测其编码氨基酸321个,属疏水蛋白,位于细胞外,信号肽位于1～18氨基酸处.同源性分析提示Der f1和Eur m1相似率为88%,而Der f1和Der p1的相似率为77%,分子进化树中粉尘螨和梅氏嗜霉螨聚成一簇.Der f1的二级结构由α-螺旋(109 aa,33.96%)、延伸链(55 aa,17.13%)、β-转角(18 aa,5.61%) 和随机卷曲(139 aa,43.30%)组成.结论 尘螨变应原Der f1原核表达获得成功,为进一步生产重组变应原奠定了基础.生物信息学分析表明粉尘螨和梅氏嗜霉螨的亲缘关系可能更近,而与屋尘螨关系稍远,此与现行的形态学分类系统并不符合.     

内蒙古白绒山羊TSC2基因克隆与表达模式分析

旨在克隆内蒙古白绒山羊TSC2基因cDNA并分析其特性及基本表达模式.利用RT-PCR分段克隆TSC2基因cDNA片段并测序,将得到的cDNA各片段核苷酸序列拼接后获得绒山羊TSC2基因编码区全长序列(HQ684023)并进行生物信息学分析.半定量RT-PCR方法检测TSC2基因在不同组织中的表达特异性.结果表明内蒙古白绒山羊TSC2基因cDNA编码区核苷酸序列为5184 bp,包含了编码1727个氨基酸残基的全长ORF.核苷酸序列与牛、猪、马、大熊猫、犬、恒河猴、人、小鼠及大鼠的同源性分别为97％、90％、89％、88％、87％、87％、87％、86％和86％.NCBI CDD程序预测该基因编码的蛋白质有一个Tuberin结构域和一个Rap-GAP结构域;Psite程序分析有5个N糖基化位点、2个cAMP和cGMP依赖蛋白激酶磷酸化位点、16个蛋白激酶C磷酸化位点、25个酪蛋白激酶磷酸化位点.PSORT程序预测其定位于胞内体膜.TSC2基因在内蒙古白绒山羊的睾丸、脑、肝脏、肺、乳腺、脾和肾脏等组织中都有表达,mRNA丰度在睾丸中较高,乳腺中较低.     

尘螨变应原Der f 1核酸序列测定及其分子进化分析

目的：对尘螨主要变应原Der f 1进行核酸序列测定,探讨其系统进化信息。方法：根据Genbank公布的Der f 1基因序列设计引物,巢式PCR扩增Der f 1的cDNA,纯化、回收、克隆至pMD19-T simple后进行序列测定,序列比对后用Clustal W1.83构建分子进化树。结果：成功扩增出Der f 1的cDNA片段,测序表明该基因含ORF1个,长度966bp,与参考序列同源性达99．9％。该变应原具半胱氨酸蛋白酶活性,与果蝇进化关系最远,与梅氏嗜霉螨进化关系最近。结论：成功获得了尘螨变应原Der f 1基因片段．根据其编码的氨基酸序列构建出的系统进化树与形态学分类不一致。     

Sequence polymorphisms of Der f 1, Der p 1, Der f 2 and Der p 2 from Korean house dust mite isolates

Amino acid sequence variations have possible influences on the allergenicity of allergens and may be important factors in allergen standardization. This study was undertaken to investigate the sequence polymorphisms of group 1 and 2 allergens from Korean isolates of the house dust mites Dermatophagoides farinae and D. pteronyssinus. cDNA sequences encoding group 1 and 2 allergens were amplified by RT-PCR and compared the deduced amino acid sequences. Der f 1.0101, which appeared in 64.0 % of the 50 sequences analyzed, was found to be predominant. Among the Der p 1 sequences, Der p 1.0102 and 1.0105 were predominant (58 %). Among the Der f 2 sequences, Der f 2.0102 (40.7 %) and a new variant with Gly at position 42 (27.8 %) were predominant. The deduced amino acid sequences of 60 Der p 2 clones were examined, and 28 variants with 1-5 amino acid substitutions were found. Interestingly, all of the Der p 2 sequences had Thr instead of Lys at position 49. Two variants (Leu40, Thr49, and Asn114 (26.6 %); Val40, Thr49, and Asn114 (20.0 %)) were found to be the most predominant forms of Der p 2. Der p 1 has a high rate of sporadic substitutions and the group 2 allergens show a more regular pattern with orderly associations of amino acid substitutions. Der f 1 and Der p 2 from Korean mite isolates have unique amino acid sequence polymorphisms. These findings provide important data for house dust mite allergen standardization.     

Antigen Der f I from the dust mite Dermatophagoides farinae: structural comparison with Der p I from Dermatophagoides pteronyssinus and epitope specificity of murine IgG and human IgE antibodies

The physicochemical and antigenic properties of an allergen purified from Dermatophagoides farinae, Der f I, were compared with Der p I from Dermatophagoides pteronyssinus. On SDS-PAGE, Der f I migrated as a single polypeptide chain with the same m.w. as Der p I (24,000). Two isoallergenic peaks of Der f I were identified on preparative isoelectric focusing (pI 5.7 to 6.3 and pI 6.6 to 6.95). Fractions from each peak were shown to have an identical amino acid composition (which was similar but not identical to Der p I) and the same N-terminal amino acid sequence. There was a good correlation between quantitative intradermal skin tests to both purified allergens and to D. farinae extract in mite-allergic patients, with positive results when using as little as 10(-5) micrograms/ml of Der f I. The majority of sera with detectable IgE antibody to D. farinae also had IgE antibody to Der f I both among children (29/42 = 69%) and adults (55/63 = 87%). By RAST, there was an excellent correlation between IgE antibody to Der f I and Der p I in sera from 42 mite-allergic children (n = 0.94, p less than 0.001). Polyclonal IgG antibodies from six mice immunized with Der f I showed preferential binding to that allergen, and most monoclonal antibodies (16 of 18) raised against Der f I did not bind Der p I. However, two monoclonal antibodies from this fusion showed cross-reactive binding to both allergens. Immunoabsorption experiments, using D. pteronyssinus and D. farinae extracts coupled to Sepharose, showed that a large proportion of murine antibodies (74% to Der p I and 60 to 93% to Der f I) could not be absorbed by the heterologous extract on the immunosorbent. In contrast, in sera from seven mite-allergic patients, most of the specific IgE and IgG antibody (i.e., greater than or equal to 82%) was removed by either immunosorbent. Thus, Der f I and Der p I represent a homologous pair of major allergens which possess both cross-reacting and species-specific epitopes. The antibody response in mice immunized with either allergen in complete Freund's adjuvant was largely directed against species-specific epitopes, whereas in allergic humans, IgE- and IgG-specific antibodies bound predominately to cross-reacting epitopes.     

Monoclonal antibodies to recombinant Der p 2, a major house dust mite allergen: specificity, epitope analysis and development of two-site capture ELISA.

House dust mite allergens have been well established as sensitizing agents that are important in the induction of allergic diseases. In order to analyze epitopes of the allergen and to develop a quantitative method of the allergen exposure, monoclonal antibodies against a recombinant Der p 2 (rDer p 2), one of the major allergens of Dermatophagoides pteronyssinus, were produced. Four monoclonal antibodies produced were species-specific and did not cross-react to the D. farinae crude extract. Two of the monoclonal antibodies were found to be IgG1 and the others were IgM. For the analysis of epitopes, a Der p 2 cDNA encoding 126 amino acids (aa) was dissected into three fragments with several overlapping peptides. A (aa residues 1-49), B (44-93), and C fragment (84-126). Three monoclonal antibodies showed reactivities to the recombinant B fragment and to the full-length rDer p 2, but one monoclonal antibody reacted only with the full-length rDer p 2. Two-site capture ELISA was developed using two different monoclonal antibodies for quantitating Der p 2 in house dust. The sensitivity limit was 4 ng/ml with rDer p 2 and 8 micrograms/ml with the D. pteronyssinus crude extract. The result suggested that the assay using monoclonal antibodies against rDer p 2 could be useful for the environmental studies and for the standardization of mite allergen extracts.     

深圳地区粉尘螨Ⅱ类变应原基因的多态性分析及其表达蛋白的变应原性鉴定

粉尘螨Ⅱ类变应原(Der fⅡ)是粉尘螨Dermatophagoides farinae主要变应原之一,可引发Ⅰ型变态反应。从深圳地区挑取活粉尘螨,经形态鉴定后纯培养,提取其总RNA,RT-PCR扩增出Der fⅡ 基因,克隆到pMD18-T载体后测序。通过计算机软件分析该基因的多态性。将该目的基因克隆到pET-His表达载体上得到重组质粒pET-Der fⅡ。工程菌经IPTG诱导培养,表达Der fⅡ目的蛋白,该蛋白主要以包涵体形式存在。重组Der fⅡ蛋白通过6His-tag蛋白纯化系统进行分离、纯化,并进行Western blot检测该重组蛋白与对粉尘螨过敏患者血清中IgE的反应性。结果表明,克隆的5株深圳地区的Der fⅡ 基因与GenBank公布的Der fⅡ(AB195580.1)核苷酸序列同源性为96.8%～99.3%,推导的氨基酸序列同源性为93.8%～98.6%。表达纯化的5种重组Der fⅡ蛋白经Western blot检测,表明都具有良好的变应原性。     

Cloning and expression of cDNA encoding the complete prepro-form of an isoform of Der f 1, the major group 1 allergen from house dust mite Dermatophagoides farinae

cDNA clones encoding a major house dust mite allergen, Der f 1, were isolated from a Dermatophagoides farinae cDNA library by plaque immunoscreening using rabbit anti-Der f 1 serum. The sequences cover the complete open reading frame encoding the prepro-form. The sequence is different from previously reported cDNA of Der f 1 in six bases and the encoded amino acid sequence is different in two residues. Pro-forms of Der f 1 and its mutant, in which the N-glycosylation motif was disrupted, expressed in Pichia pastoris were converted to the mature forms by an in vitro activation process and they showed significant IgE-binding. The biologically active rDer f 1 molecules would be useful for diagnostic testing and allergen-specific immunotherapy. In contrast, Der f 1 directly expressed in Escherichia coli without the prosequence had very low IgE binding. The hypoallergenic Der f 1 polypeptide could be useful for safer and more effective immunotherapy.     

Structure of the house dust mite allergen Der f 2: implications for function and molecular basis of IgE cross-reactivity

The X-ray structure of the group 2 major allergen from Dermatophagoides farinae (Der f 2) was determined to 1.83 A resolution. The overall Der f 2 structure comprises a single domain of immunoglobulin fold with two anti-parallel beta-sheets. A large hydrophobic cavity is formed in the interior of Der f 2. Structural comparisons to distantly related proteins suggest a role in lipid binding. Immunoglobulin E (IgE) cross-reactivity between group 2 house dust mite major allergens can be explained by conserved surface areas representing IgE binding epitopes.     

尘螨变应原Derf1核酸序列测定及其分子进化分析

目的:对尘螨主要变应原Der f1进行核酸序列测定,探讨其系统进化信息。方法:根据Genbank公布的Der f1基因序列设计引物,巢式PCR扩增Der f1的cDNA,纯化、回收、克隆至pMD19-T simple后进行序列测定,序列比对后用Clustal W 1.83构建分子进化树。结果:成功扩增出Der f1的cDNA片段,测序表明该基因含ORF1个,长度966bp,与参考序列同源性达99.9%。该变应原具半胱氨酸蛋白酶活性,与果蝇进化关系最远,与梅氏嗜霉螨进化关系最近。结论:成功获得了尘螨变应原Der f1基因片段,根据其编码的氨基酸序列构建出的系统进化树与形态学分类不一致。     

The binding of mouse hybridoma and human IgE antibodies to the major fecal allergen, Der p I, of Dermatophagoides pteronyssinus. Relative binding site location and species specificity studied by solid-phase inhibition assays with radiolabeled antigen

The relative binding site location and species specificity of 19 mouse hybridoma antibodies, produced in four laboratories, to Dermatophagoides pteronyssinus major fecal allergen, Der p I, was studied by using immobilized mAb and inhibitions of radiolabeled Ag binding. Four mAb groups were defined, within which 4, 6, 8, and 5 mAb, respectively, cross-inhibited each other. Five mAb were members of both group 2 and 3, demonstrating a considerable overlap of epitopes between the corresponding antibody-binding regions. The degree of mAb species specificity, as assessed by inhibition with cold Der p I and Ag Der m I and Der f I from the related species, Dermatophagoides microceras and Dermatophagoides farinae, was highly variable even for mAb binding to the same region on the Ag. Five cases of cross-reactivity between Der p I and Der m I and one case of cross-reactivity between Der p I and Der f I were found. The N-terminal 30 amino acids of the three species showed 7 substitutions between Der p I and Der m I/Der f I and 2 between Der f I and Der p I/Der m I. Single mAb inhibited up to 65% of labeled Der p I binding to immobilized human IgE from allergic patients' sera and up to 24% of labeled Der p I binding to immobilized rabbit antibodies. The spectrum of species specificities in human IgE sera, as assessed by inhibitions with cold Ag, was similar to that of the mAb. No evidence for the presence of strictly sequential epitopes, reactive with either mAb or human IgE was found, as judged from the weak inhibitory activity of acid-denatured Der p I.     

Nuclear magnetic resonance structure-based epitope mapping and modulation of dust mite group 13 allergen as a hypoallergen

IgE-mediated allergic response involves cross-linking of IgE bound on mast cells by specific surface epitopes of allergens. Structural studies on IgE epitopes of allergens are essential in understanding the characteristics of an allergen and for development of specific allergen immunotherapy. We have determined the structure of a group 13 dust mite allergen from Dermatophagoides farinae, Der f 13, using nuclear magnetic resonance. Sequence comparison of Der f 13 with homologous human fatty acid-binding proteins revealed unique surface charged residues on Der f 13 that may be involved in IgE binding and allergenicity. Site-directed mutagenesis and IgE binding assays have confirmed four surface charged residues on opposite sides of the protein that are involved in IgE binding. A triple mutant of Der f 13 (E41A_K63A_K91A) has been generated and found to have significantly reduced IgE binding and histamine release in skin prick tests on patients allergenic to group 13 dust mite allergens. The triple mutant is also able to induce PBMC proliferation in allergic patients with indices similar to those of wild-type Der f 13 and shift the secretion of cytokines from a Th2 to a Th1 pattern. Mouse IgG serum raised using the triple mutant is capable to block the binding of IgE from allergic patients to wild-type Der f 13, indicating potential for the triple mutant as a hypoallergen for specific immunotherapy. Findings in this study imply the importance of surface charged residues on IgE binding and allergenicity of an allergen, as was also demonstrated in other major allergens studied.