油桐尺蠖核型多角体病毒多角体蛋白的理化性质及二级结构预测

由ＳＤＳ及梯度胶电泳测得测得油桐尺蠖核型多型多角体病毒多角体蛋白天然状态及亚基分子量分别为３６３ｋＤ与３１．５ｋＤ从而推断此蛋白为十二聚体,亚基间无二硫键作用,ＢｓＮＰＶ多角体蛋白的远紫外圆二色谱显示,它的二级结构含有３１．７％的α螺旋,２３．８％的β折叠及４４．５％的无规卷曲,与二级结构预测结果相符,通过荧光光谱实验推知,ＢｓＮＰＶ多角体蛋白的表面疏水性弱;其色氨酸残基位于蛋白疏水核内部。     

昆虫病毒多角体蛋白基因的克隆及其在大肠杆菌中的表达

将含有大尺蠖核型多角体病毒(BsNPV)多角体蛋白基因(ocu)的BamHl一H片段克隆到表达载体pDR 540的BamiHl位点,得到能抗高浓度氨苄青霉素(200μg／ml)的两个阳性重组体,其胞外总蛋白比亲本质粒高1．1-1．4倍。在大肠杆菌细胞中,BsNPV ocu基因在原核杂合启动子tac驱动下能高水平的表达,表达量达到0．8和4．7mg／ml。免疫沉淀反应证明,表达蛋白为BsNPV的包涵体蛋白,凝胶过摅法测定的平均分子量为32.1×103道尔顿。     

粘虫核型多角体病毒多角体蛋白基因结构和序列的研究

测定了粘虫核型多角体病毒（Ｌｅｕｃａｎｉａｓｅｐａｒａｔａｎｕｃｌｅａｒｐｏｌｙｈｅｄｒｏｓｉｓｖｉｒｕｓ,ＬｓＮＰＶ）两个ＥｃｏＲＶ片段的共１２０１ｂｐ序列,发现了一个７１４ｂｐ的开放阅读框（ＯＲＦ）,根据其与多种ＮＰＶ多角体蛋白基因（ｏｃｕ）同源性的比较和５＇端典型的１４ｂｐ保守序列,说明此ＯＲＦ即为ＬｓＮＰＶ的ｏｃｕ基因。根据核苷酸序列预测的多角体蛋白有２４６个氨基酸,其中酸性和碱性氨基酸数相等,疏水氨基酸含量很高,氨基酸组成中以谷氨酸（Ｇｌｕ）含量最高,谷氨酰胺和半胱氨酸含量最低。编码区碱基同源性与ＭｂＮＰＶ最高,为９７．０％;氨基酸同源性与ＭｂＮＰＶ最高,为９７．５％。密码子偏爱选用以第三个碱基为嘧啶的密码子。二级结构分析表明,α－螺旋（Ｈ）和β－折叠（Ｓ）相等,β－转角含量是Ｈ和Ｓ含量之和。     

大尺蠖核型多角体病毒多角体蛋白基因的结构分析

大尺蠖核型多角体病毒(BsNPV)的多角体蛋白基因(ocu)定位在2．3kb的BamHl—H片段上,用xho1、sma1、HindIII和PstI构建了H片段的物理图谱,并测定了两端636bp序列。在5’端发现了杆状病毒ocu基因共有的典型特征,即：ATG起始区;启动子区(14bp保守序列);TATA box和CATA box区等。单一xhoI位点在ATG上游-15bp处,适于作为构建ocu基因转移载体的插入位点。在这一基因5’端序列中发现了五个反转重复单元CGAGC GCTCG,讨论了这一单元在杆状病毒ocu基因高效表达中的调控功能。     

多角体蛋白的结构多样性和杆状病毒的进化研究

在测定ＬｓＭＮＰＶ多角体蛋白基因的全序列并推导出多角体蛋白氨基酸顺序的基础上,与２２种杆状病毒多角体蛋白的氨基酸顺序进行比较,以氨基酸变异曲线研究蛋白质一级结构中氨基酸的保守性,并推测一个模式多角体蛋白（ＭＰｈ）氨基酸顺序;用ＰＲＯＳＩＳ软件对ＭＰｈ及其它５种代表性病毒的多角体蛋白进行了氨基酸亲水性分析,还对２４种多角蛋白的二级结构作出了推测,指出了特征性结构区与氨基酸高变区,亲水区多样性变化的相     

油桐尺蠖核多角体病毒多角体蛋白基因定位与克隆

以[~(32)P]-dATP标记含AcNPV DNA的EcoRI-I片段的重组质粒为探针,在35℃条件下对油桐尺蠖核多角体病毒(BsNPV)多角体蛋白基因进行了定位,将其分别定位在BamH Ⅰ-A,Bgl Ⅰ-A,Bgl Ⅱ-F,EocR Ⅰ-R,Hind Ⅲ-A,Kpn Ⅰ-Ⅰ,Pst Ⅰ-D,Xba Ⅰ-A(或B),Xho Ⅰ-F和G片段上,并以M13mp18为载体,克隆了Kpn Ⅰ-Ⅰ片段。     

异源多角体蛋白对家蚕核型多角体病毒粒子的包装

利用PCR方法从AcMNPV基因组DNA中分离出多角体蛋白基因 ,将该扩增片段克隆到转移载体pBacPAK8中 ,得到重组转移载体pOAc。将该质粒DNA与线性化的Bm BacPAK6病毒基因组DNA共传染BmN细胞 ,得到了能形成多角体且不产生蓝色空斑的重组病毒hp BmNPV。纯化该重组病毒的多角体颗粒 ,并对多角体蛋白、病毒核酸及多角体病毒颗粒进行分析 ,发现AcMNPV的多角体蛋白能在家蚕细胞中大量表达且能在细胞内识别家蚕核型多角体病毒并组装成多角体颗粒 ;病毒基因组DNA因部分交换 ,其酶切行为发生了相应的变化 ;电镜观察发现经AcMNPV多角体蛋白包装的家蚕核型多角体病毒的多角体颗粒大小为1 2 μm～ 2 9μm ,明显小于野生型家蚕核型多角体病毒的多角体颗粒     

茶尺蠖核型多角体病毒多角体蛋白单克隆抗体的制备

为了建立一种基于免疫反应检测茶尺蠖核型多角体病毒的方法,以纯化后的茶尺蠖核型多角体病毒作为抗原,免疫BALB/c小鼠,将小鼠脾脏细胞与小鼠骨髓瘤细胞Sp2/0融合,经间接ELISA筛选及克隆得到了一株稳定分泌单克隆抗体的杂交瘤细胞株,命名为7D3。同时克隆并在大肠杆菌中表达了EoNPV多角体蛋白基因,获得重组多角体蛋白。经Western blotting鉴定,该抗体可与EoNPV的多角体蛋白特异性结合。利用制备EoNPV多角体蛋白的单克隆抗体,建立了间接ELISA测定EoNPV的方法。     

原位化学切割法对油桐尺蠖核型多角体病毒两种相似多肽的比较研究

油桐尺蠖核型多角体病毒(BsNPV)自1978年分离以来,对其形态结构、形态发生、毒力测定、血清学、理化特性、安全性试验、剂型研究及大田应用等已进行了广泛的研究,其基因组物理图谱也已构建。采用SDS-聚丙烯酰胺凝胶电泳(SDS-PAGE)研究BsNPV蛋白质时发现,多角体蛋白与病毒粒子的一种主要蛋白质的分子量非常接近,     

银染色测定粘虫核多角体病毒多角体基因序列

LsMNPV DNA用EcoRV酶切进行基因组克降,用AcMNPV的部分多角体基因顺序DNA片段作探针,菌落原位杂交法结合测序筛选到分别含LsMNPV部分多角体基因的重组质粒pLsEV1和pLsPH5。用银染色PCR线性扩增双脱氧法测序,发现LsMNPv的完整基因即位于这两个片段上。LsMNPV多角体基因长741bp,编码区碱基同源性与AcMNPV和MbMNPV分别为80.0％和97.0％,氨基酸同源性分别为89.8和97.5％。氨基酸组成中以谷氨酸(Glu)含量最高,谷氨酰胺和色氨酸含量最低。密码子选用以第三个碱基为嘧啶的密码子频率最高。多角体蛋白N端有一类似信号肽结构的26个氨基酸的疏水区。     

蚕豆蛋白质亚基分析与特异种质鉴定

采用SDS-PAGE方法,对112份不同基因型蚕豆的清蛋白和球蛋白亚基的差异性进行分析。结果显示:(1)蚕豆清蛋白和球蛋白亚基的有效等位变异分别为1.750 0±0.452 3、1.545 5±0.522 2,多态性比率分别为75.00%、54.55%,清蛋白的亚基遗传多样性指数较球蛋白亚基高。(2)蚕豆清蛋白和球蛋白分别含有在不同基因型蚕豆中构成不同的12和10个亚基,其中清蛋白含有9个基本亚基,116kD、96kD、45kD为清蛋白的3个特异亚基;球蛋白含有8个基本亚基,58kD、35kD为球蛋白的2个特异亚基;研究共鉴定筛选出42个含有清蛋白特异亚基和21个含有球蛋白亚基的种质资源。(3)清蛋白的97kD、63kD基本亚基和球蛋白的97kD、56kD、47kD基本亚基存在一定的缺失现象,共鉴定出19个清蛋白亚基和21个球蛋白亚基缺失的优异种质。研究表明,蚕豆清蛋白和球蛋白亚基构成在不同种质之间具有差异性,除基本亚基外,部分种质还含有特异亚基或缺失亚基。     

花生种子发育和萌发过程中贮藏蛋白的合成和降解

以花生品种汕油5 2 3种子为材料,分离纯化花生球蛋白的41 kD和38.5 kD两种主要亚基及伴花生球蛋白的6 0.5 KD亚基并制备抗体.We stern blot分析表明,3种亚基在花生胚组织分化期的胚轴和子叶中就开始合成,其中60.5 kD亚基是最先在胚轴和子叶中大量合成和积累的贮藏蛋白,41 kD和38.5 kD亚基在随后的发育中积累量不断增加;种子萌发时这3种亚基的降解进程不一样,胚轴和子叶中41 kD和38.5kD亚基的降解均先于60.5 kD亚基.     

14-3-3 Protein homologues play a central role in the fusicoccin signal transduction pathway

The plasma membrane located fusicoccin binding protein (FCBP) is an essential element in the fusicoccin (FC) signal transduction pathway. We obtained primary sequence information for the 31 kD subunit of the FCBP. These sequences showed that the FCBP is homologous to members of the 14-3-3 protein family. Both the 31 and 30 kD subunits cross-react with 14-3-3 antibodies. In native form the FCBP occurs as a dimer, but it is also part of a complex with higher molecular mass. The monomeric forms of the FCBP (the 30 and 31 kD subunits) do not have ³H-FC binding activity. We discuss how the FCBP, as a member of the 14-3-3 protein family, may be able to bind FC and how the FC-signal is transduced to the effector protein, the H⁺-ATPase.     

牛脑液泡型质子泵70kD和33kD亚基基因的表达

已分离了编码牛脑液泡型质子泵的70kD亚基的cDNA,利用聚合酶链反应(PCR)扩增了70kD亚基的编码片段,同时直接从牛脑cDNA库中得到了33kD亚基的编码片段.分别将相应片段连接到PET载体上完成70kD和33kD亚基基因在大肠杆菌中的表达.SDS聚丙烯酰胺凝胶电泳和蛋白质印迹分析表明70kD和33kD亚基基因均得到明显表达.     

Analysis of genes coding for the sialic acid-binding adhesin and two other minor fimbrial subunits of the S-fimbrial adhesin determinant of Escherichia coli

The S fimbrial adhesin (Sfa) enables Escherichia coli to attach to sialic acid-containing receptor molecules of eukaryotic cells. As previously reported, the genetic determinant coding for the Sfa of an E. coli O6 strain was cloned, the gene coding for the major fimbrial subunit was identified and sequenced and the S specific adhesin was detected. Here we present evidence that in addition to the major subunit protein SfaA three other minor subunit proteins, SfaG (17 kD), SfaS (14 kD) and SfaH (31 kD) can be isolated from the S-specific fimbrial adhesin complex. The genes coding for these minor subunits were identified, mutagenized separately and sequenced. Using haemagglutination tests, electron-microscopy and quantitative ELISA assays with monoclonal anti-SfaA and anti-SfaS antibodies the functions of the minor subunits were determined. It was determined that SfaS is identical to the S-specific adhesin, which also plays a role in determination of the degree of fimbriation of the cell. The minor subunit SfaH also had some influence on the level of fimbriation of the cell, while SfaG is necessary for full expression of S-specific binding. It was further shown that the amino-terminal protein sequence of the isolated SfaS protein was identical to the protein sequence calculated from the DNA sequence of the sfaS gene locus.     

莲子贮存蛋白的主要亚基及积累模式

红莲（NelumbonuciferaGaertn）成熟于叶总蛋白含量达24．35g／100g干样品,其贮存蛋白（SP）的积累模式与豆科种子相似,即随成熟度的提高,SP猛增至占总蛋白含量的86％以上。对莲子不同发育阶段子叶蛋白SDS-PAGE图谱的光密度测定表明：莲子叶蛋白有12个主要SP亚基（SP1－12）。按分子量（MW）大小和积累顺序可分3组：A组是98kD和93kD的2个亚基,MW最大,积累最晚,但量最多;B组是3个亚基,MW为55－50kD,大小居中,积累最早,量最少;C组的7个亚基MW最小,在27－14kD之间,积累较早,量较多。对莲的不同品种、不同器官进行分析后发现,它们都有1个主峰为68kD的多连峰的代谢蛋白亚基,可能是莲共有的蛋白亚基。     

野桑蚕卵黄原蛋白的鉴定及cDNA序列分析

利用SDS-PAGE和Western blot方法分析鉴定了野桑蚕Bombyx mandarina Moore卵黄原蛋白,发现该蛋白由大小两个亚基组成,分子量分别为175 kD和42 kD。利用昆虫卵黄原蛋白进化上的保守性,根据家蚕的卵黄原蛋白cDNA序列设计特异性引物在野桑蚕的总RNA进行RT-PCR扩增,对于3′和5′端进行RACE扩增,解析获得了野桑蚕卵黄原蛋白cDNA全序列(GenBank登录号AY 309967)。该序列含有5.754个碱基,由一个开放阅读框组成,编码1.780个氨基酸,卵黄原蛋白的氨基酸序列与家蚕的同源性达到97.6%。在特定的酶切位点(RSRR)处,即第364～367个氨基酸位置,卵黄原蛋白前体被酶切为大小两个亚基,根据氨基酸推算的相对分子质量分别为161.571 kD和40.794 kD,如果考虑到翻译后的修饰,这与SDS-PAGE的结果是吻合的。同源性分析表明,昆虫卵黄原蛋白一级结构分化基本上局限在同一目内,具有较高的保守性。     

Isolation and characteristics of dihydropyridine calcium antagonist receptor from rabbit skeletal muscles

Up to 80% of the dihydropyridine receptor is solubilized from transverse tubules of rabbit skeletal muscle by 3-[(3-cholamidopropyl)-dimethylammonium]-2-oxy-1-propane sulfonate (CHAPSO). The DHP receptor is an oligomeric complex made up of two subunits with molecular masses of 160 and 53 kD as shown by DHP-Sepharose affinity chromatography and SDS gel electrophoresis of specifically eluted proteins. The reduction of disulfide bridges of the 160 kD subunit is accompanied by a decrease in its apparent molecular mass up to 125 kD. A method is proposed for preparative isolation of the DHP receptor which is based on ion-exchange chromatography and WGA-Sepharose chromatography. Individual subunits of DHP receptor were isolated by Sepharose 4B gel filtration in SDS; their amino acid composition was determined. Both the 160 and 53 kD subunits are N-glycosylated, and the oligosaccharide portions make up to 7.5% and 6.6%, respectively.     

红苋R104种子谷蛋白的电泳分析

通过单向水平变性聚丙烯酰胺凝胶等电聚焦（ＩＥＦ）、十二烷基硫酸钠聚丙烯酰胺凝胶电泳（ＳＤＳ—ＰＡＧＥ）和双向电泳（ＩＥＦ×ＳＤＳ—ＰＡＧＥ）分析了红苋Ｒ１０４种子谷蛋白的亚基组成,亚基分子量和等电点分布。谷蛋白的双向电泳图谱可分辨出１００多个亚基成分．其主要亚基为：５４ｋＤ（ｐＩ７．１５）;３３ｋＤ（ｐＩ５．８２）;３１ｋＤ（ｐＩ６．９２;ｐＩ６．７０;ｐＩ６．６５）;２２ｋＤ（ｐＩ８．３４）;２０ｋＤ（ｐＩ６．９２;ｐＩ６５６）;１８ｋＤ（ｐＩ６．９２;ｐＩ７３５;ｐＩ７．７２;ｐＩ８．０５）。另外,还对ＩＥＦ方法进行了讨论。     

Ca2+/calmodulin-dependent protein phosphatase in bovine parotid gland: purification and characterization

Calmodulin-dependent protein phosphatase (CaM-PPase) was isolated from bovine parotid gland by sequential application of DEAE-52, Affi-gel blue and calmodulin-affinity chromatography followed by gel filtration and high performance liquid chromatography. The enzyme was activated in the simultaneous presence of Ni2+ or Mn2+ and Ca2+ plus calmodulin. Ca2+/calmodulin-dependent activation of CaM-PPase was antagonized by inhibitors of calmodulin action, such as W-7 and trifluoperazine. Tryptophan fluorescence was quenched in the presence of Ni2+. CaM-PPase was a heterodimer. The molecular weights of large subunits which bound calmodulin (CaM) were 68 kD and 58 kD - the 68 kD subunit was predominant. Polyclonal antibodies against bovine calcineurin cross-reacted with both types of larger subunits. Using polyclonal antibodies against bovine calcineurin or the monoclonal antibody against subunit B of bovine calcineurin, the smaller molecular weight subunit (19 kD) was found to be immunologically identical to subunit B of bovine calcineurin. In bovine parotid gland, CaM-PPase was found both in acinar and duct cells.