北极狐γ-干扰素cDNA的克隆、表达及活性测定

为研究狐γ-干扰素的生物学活性,应用反转录聚合酶链式反应(RT-PCR)从北极狐外周血淋巴细胞中扩增出γ-干扰素(VuIFN-γ)cDNA.序列分析表明VuIFN-γcDNA全长501 bp,编码23个氨基酸的信号肽和144个氨基酸的成熟肽蛋白,与已发表的银黑狐和犬IFN-γ核苷酸序列同源性为99.8%和99.4%;氨基酸同源性均为100%.应用原核表达系统高效表达北极狐γ-干扰素成熟肽蛋白,SDS-PAGE和Western blotting分析表达的融合蛋白分子量约为19 kD,以不溶性的包涵体形式存在.重组蛋白经纯化和复性,在Vero和MDCK细胞上可明显抑制VSV病毒的复制,并测出北极狐重组γ-干扰素的活性单位分别为1.0×106 u/mg和1.56×105 u/mg,为进一步开发基因工程狐干扰素奠定基础.     

重组马g-干扰素抗病毒活性测定及单克隆抗体抑制活性鉴定

为了测定大肠杆菌和杆状病毒表达的重组马g-干扰素是否具有抗病毒活性, 利用这两种干扰素处理马胎肾细胞(EFK-78), 然后接种表达绿色荧光蛋白(GFP)的重组水泡性口炎病毒(VSV*GFP), 观察干扰素对病毒表达GFP的抑制, 测出其抗病毒活性单位分别为1×103 AU/mL、1×105 AU/mL。评价了制备的九株抗重组马g-干扰素单克隆抗体是否可抑制重组马g-干扰素抗病毒活性, 证实其中一株可中和重组马g-干扰素的抗病毒活性。结果表明: 杆状病毒表达的马g-干扰素具有较高的抗病毒活性, 其活性可被一株制备的抗重组马g-干扰素单克隆抗体抑制; 首次获得原核表达的具有抗病毒活性的马g-干扰素。     

奶牛γ干扰素基因的高效表达及活性测定

经刀豆素(conA)刺激诱导奶牛外周血淋巴细胞,应用RT-PCR方法从其总RNA中对奶牛γ干扰素基因cDNA进行扩增,然后将特异性片段连接到pMD18-T载体,测序结果表明,与已知序列同源性为100%.然后将特异性片段连在pRLC载体上进行表达,经SDS-PAGE分析,原核表达产物为16kDa的重组蛋白,占菌体总蛋白的42%,表达产物以包涵体形式存在.经7mol/L盐酸胍的变性液溶解及0.5mol/L盐酸胍复性液处理,表达产物进行脱盐、凝胶层析纯化,细胞病变抑制法结果表明,重组牛IFN-γ具有较高的干扰素活性,约为6.0×105U/mg.     

北极狐GHR基因cDNA的克隆及序列分析

本文根据狗(AF133835)的GHR基因cDNA编码全序列设计了三对引物,利用RT-PCR方法克隆出北极狐GHR基因编码区全长cDNA序列(GenBank accession No.EU304325)。结果表明,北极狐GHR的ORF为1917bp,编码638个氨基酸的前体蛋白,由18个氨基酸的信号肽和620个氨基酸的成熟肽组成。通过同源性比较发现北极狐与狗的同源性最高,达到98%。另外,利用邻接法(NJ法)构建的分子系统进化树聚类结果表明,北极狐与狗先聚为一类,该聚类结果与传统的物种进化关系基本一致。另外,通过氨基酸对位序列比较发现,北极狐GHR在氨基酸序列上存在明显的特异性,如45和451位分别为A和E,而其它物种均分别为T(大鼠为K)和A(牛羊为V,鼠为T)。     

重组鲁西黄牛α干扰素融合蛋白的表达及其抗病毒活性研究

通过PCR从鲁西黄牛(Yellowcattle)基因组DNA中克隆了α干扰素(BoIFN-α)基因,并插入到pET32a 中,构建成重组原核表达质粒pET32a /BoIFN-α,进行测序和诱导表达。测序结果表明,鲁西黄牛IFN-α基因全长498个核苷酸,含一个开放阅读框(ORF),编码166个氨基酸的成熟蛋白,与已报道的牛α干扰素C亚型氨基酸组成同源性为97.6%。表达产物经SDS-PAGE分析,表达出40kD的融合蛋白,表达量占菌体总蛋白的26.7%。表达产物经镍离子螯合次氨基三乙酸(Ni-NTA)亲和层析纯化,纯化产物进行复性后在MDBK/VSV上的活性为5×105u/mg。重组牛IFN-α(rBoIFN-α)对牛轮状病毒(BRV)有一定的抑制作用,抗BRV病毒活性为1.5×105u/mg。结果显示从鲁西黄牛中克隆了IFN-α基因的一种新亚型,即BoIFN-αC2,并实现了高效表达,获得了具有较高抗病毒活性的重组干扰素产物,为重组牛干扰素的开发奠定了基础。     

中华蜜蜂蜂毒镇静肽基因的cDNA克隆和表达

从中华蜜蜂 (Apisceranacerana)工蜂毒腺中快速抽提总RNA ,用RT PCR扩增得到大小约为2 5 0bp的cDNA片段 ,测序得到的片段长度为 2 34bp ,为蜂毒前镇静肽原 (preprosecapin)基因编码区的cDNA .以 3′RACE方法 ,扩增和测定了 3′端非编码区 2 19bp序列 .中蜂前镇静肽原cDNA序列与已报道的欧洲意蜂该基因cDNA序列具有 92 %同源性 ,氨基酸序列具有 87%同源性 .代表成熟肽镇静肽的最后 2 5个氨基酸序列 ,中蜂与意蜂同源性为 88% .3′端非编码区cDNA序列与欧洲意蜂序列有 73 1%同源性 .将中华蜜蜂蜂毒镇静肽成熟肽编码区与 3′非编码区部分克隆 ,构建了镇静肽与谷胱甘肽转移酶融合表达的载体pGEX AcSecapin .将载体转化大肠杆菌BL2 1(DE3)进行融合表达 .表达产物与抗GST抗体在 2 9kD处有很强的交叉反应 .大肠杆菌超声破碎后的上清液用SDS PAGE检测到表达的蛋白多为可溶性融合蛋白 ,通过亲和层析柱纯化和凝血酶的切割得到了镇静肽蛋白     

重组人α2a干扰素的高效表达与纯化

构建了人α2a型干扰素的表达载体,并在大肠杆菌中获得了高效表达,表达量平均为10~ IU/L菌液。还对其表达产物进行了纯化。经盐酸胍裂解菌体、硫酸铵沉淀、酸化处理,再经阴、阳离子交换层析和单克隆抗体亲和层析,使表达产物纯化了1072倍,比活性达1.2×IO~ IU/mg蛋白,达到序列纯,回收率达54％。表达产物N端21个氨基酸序列分析结果与IFN-α2a cDNA推导的序列相符合。     

人Artemin cDNA扩增及表达

以人胎脑RNA为模板, 采用RT-PCR技术扩增人Artemin cDNA。序列分析表明, 扩增的人Artemin cDNA核苷酸序列与已发表序列(GenBank登录号：AF115765)同源性为99.7%, 氨基酸序列同源性为100%。将经过序列分析确定的Artemin cDNA插入原核表达载体pGEX-6p-1中, 构建重组表达载体pGEX-6p-1-hART。通过SDS-PAGE分析重组人Artemin融合蛋白在大肠杆菌中的表达情况。结果表明, 重组人Artemin融合蛋白表达量约占宿主菌总蛋白的18.32%, 主要以包涵体形式存在。对表达的重组人Artemin融合蛋白包涵体进行溶解和复性, 并进行Western blotting分析。说明体外成功扩增人Artemin cDNA, 并在原核表达系统中高效表达了重组人Artemin融合蛋白。     

家兔精子膜蛋白rsp10基因的克隆和特征分析

 sp10基因在精卵识别过程中起着重要作用 .从家兔睾丸cDNA文库中克隆了家兔的sp10基因 (rsp10 ) ,cDNA序列全长 12 82bp ,包含 10 0 5bp开放阅读框 .由开放阅读框推测出的氨基酸序列与人、狒狒、狐和小鼠的SP10氨基酸序列之间存在较高水平的同源性 ,同源性分别为 70 %、69%、68%和 61% .在大肠杆菌中表达rsp10基因 ,获得重组rSP10 .用重组rSP10免疫雌性母兔 ,得到rSP10专一性多抗 .对精子膜蛋白进行免疫印迹分析发现 ,rsp10基因在家兔睾丸中的表达呈现多态性 .rsp10基因在GenBank的登录号为 :AF2 51558.     

干扰素-tau的原核表达、纯化和活性测定

干扰素-tau (IFN-tau)是一种新发现的I型干扰素,为了更清楚的研究它的生物学功能,在已克隆IFN-tau cDNA的基础上,PCR扩增出IFN-tau ORF,与原核表达载体pBV220重组后,成功的构建了IFN-tau的原核表达质粒pBV220/IFN-tau。重组质粒转化大肠杆菌BL21,该菌经过诱导,用凝胶过滤色谱层析的方法获得了纯化的目的蛋白,该蛋白经过氨基酸序列分析证实是IFN-tau ;用细胞病变抑制法测定IFN-tau经过透析复性后的活性为2.09×106IU/ml,比活性为2.35×106IU/mg。     

Expression of a biologically active ovine trophoblastic interferon using a baculovirus expression system.

Ovine trophoblast protein (oTP) an embryonic interferon, which plays a key role in maternal recognition of pregnancy, has been expressed in insect cells using a baculovirus expression system. A cDNA coding for oTP was inserted downstream of the strong polyhedrin promoter. Cells infected with recombinant virus produced biologically active oTP and greater than 90% was secreted into the culture medium during infection. High amount of antiviral activity were produced (up to 5 x 10(5) IU per ml of culture medium). Recombinant oTP (roTP) was purified by immunoaffinity chromatography and found to be identical to authentic oTP with respect to molecular mass and N-terminal amino acid sequence.     

Ribosome-inactivating activity and cDNA cloning of antiviral protein isoforms of Chenopodium album

We have characterized a novel type I ribosome-inactivating protein (CAP30) from the leaves of Chenopodium album. Purified native CAP30 depurinated the ribosomes of Chenopodium, tomato, and tobacco leaves in vitro. To further characterize this protein, cDNA clones were isolated from a leaf cDNA library using a DNA probe derived from the N-terminal amino acid sequence. Two full-length cDNA clones, CAP30A and CAP30B, were isolated. The two clones were highly homologous (91.4% identity over 280 amino acids) at the deduced amino acid level. Both contain a putative signal peptide of 25 amino acid and a conserved domain commonly found in ribosome-inactivating proteins. This suggests that CAP30 is a single-chain ribosome-inactivating protein. Expression of CAP30 mRNA peaked twice, at 12 and 72 h, after tobacco mosaic virus (TMV) infection or wounding. Transformed Escherichia coli cells expressing pre- or mature CAP had greatly reduced growth rates. These results suggest that CAP30 functions as a broad-spectrum defense-related protein with both antiviral and anti-microbial activity.     

Molecular cloning and functional identification of a ribosome inactivating/antiviral protein from leaves of post-flowering stage of Celosia cristata and its expression in E. coli

A full-length cDNA clone, encoding a ribosome inactivating/antiviral protein (RIP/AVP) was isolated from the cDNA library of post-flowering stage of Celosia cristata leaves. The full-length cDNA consisted of 1015 nucleotides, with an open reading frame encoding 283 amino acids. The deduced amino acid sequence had a putative active site domain conserved in other ribosome inactivating/antiviral proteins (RIPs/AVPs). The coding region of the cDNA was amplified by polymerase chain reaction (PCR), cloned and expressed in Escherichia coli as recombinant protein of 72 kDa. The expressed fusion product was confirmed by Western analysis and purification by affinity chromatography. Both the recombinant protein (reCCP-27) and purified expressed protein (eCCP-27) inhibited translation in rabbit reticulocytes showing IC50 values at 95 ng and 45 ng, respectively. The native purified nCCP-27 has IC50 at 25 ng. The purified product also showed N-glycosidase activity towards tobacco ribosomes and antiviral activity towards tobacco mosaic virus (TMV) and sunnhemp rosette virus (SRV).     

复合干扰素突变体在毕赤酵母中的表达、纯化及活性分析

根据毕赤酵母密码子偏性合成了复合干扰素突变体基因 ,克隆至分泌型酵母表达载体pMEX9K ,将重组载体pMEX CIFNm用SacⅠ线性化后 ,转化毕赤酵母GS115 .转化子经诱导后 ,培养上清有抗病毒活性的蛋白产生 .经过离子交换 ,疏水层析 ,凝胶过滤三步层析纯化 ,得到了纯度大于95 %的重组复合干扰素突变体 ,经N端氨基酸序列分析表明 ,该蛋白N端序列与理论值一致 ,质谱测定分子量为 19 3kD ,与理论值一致 .用细胞病变抑制法测定其活性 ,并结合Lowry法蛋白定量计算其比活性为 6× 10 8IU mg ,与复合干扰素的比活相当 .     

重组酵母鸡γ干扰素的抗病毒活性测定及临床初步应用

为了获得具有天然抗病毒活性的重组酵母鸡γ干扰素,以Con A(刀豆素A)诱导培养4~10h的鸡全血中提取的淋巴细胞总RNA为模板,通过RT-PCR的方法扩增出鸡γ干扰素成熟蛋白基因。通过EcoRⅠ和XbaⅠ两个酶切位点把鸡γ干扰素成熟蛋白基因插入到酵母表达载体pPICZa-A上,得到了重组酵母鸡γ干扰素表达载体pPICZa-A-CHIFN-γ,经BstxⅠ线性化后的重组载体被转入酵母菌株X33中,通过PCR的方法来筛选重组酵母菌,在甲醇诱导表达后,SDS-PAGE结果显示有两株重组菌在诱导72h后其表达上清中有大小为16kDa的目的条带。干扰素生物活性测定经典实验(微量病变抑制实验)和临床初步应用结果皆说明重组酵母鸡γ干扰素具有较强的抗病毒的生物活性和较好的临床使用前景。     

Molecular cloning of a cDNA encoding chicken T-protein of the glycine cleavage system and expression of the functional protein in Escherichia coli. Effect of mRNA secondary structure in the translational initiation region on expression.

DNA clones encoding chicken T-protein of the glycine cleavage system were isolated from chicken liver lambda gt10 cDNA libraries. Three overlapping clones provided an open reading frame of 1176 nucleotides that predicts a polypeptide of 392 amino acids (M(r) 42,056) comprised of a 16-residue mitochondrial targeting sequence and a 376-residue mature protein (M(r) 40,292). The amino acid sequence predicted for the mature protein showed 67% identity with that of bovine T-protein. A cDNA encoding mature T-protein was constructed, and the nucleotide sequence just downstream of the initiation codon was modified without amino acid substitution to reduce the free energy of formation for the folded mRNA. Expression plasmids containing these cDNA variants produced large amounts of T-protein in Escherichia coli, while very low expression was observed with a plasmid containing wild type cDNA. Enzymatically active T-protein was obtained when the expression was conducted at 30 degrees C with 25 microM isopropyl-1-thio-beta-D-galactopyranoside. Under the full inducing condition (at 37 degrees C and 1 mM inducer), the expressed T-protein was recovered as insoluble and inactive protein. The recombinant T-protein was purified to near homogeneity with a yield of about 30%. Apparent molecular weight on sodium dodecyl sulfate-polyacrylamide gel electrophoresis is approximately 40,000, similar to the size of T-protein purified from chicken liver. NH2-terminal amino acid sequence analysis (9 residues) revealed 100% identity with chicken T-protein determined chemically. The kinetic properties of the recombinant T-protein resembled those of the native chicken T-protein.     

Molecular cloning of feline interferon cDNA by direct expression.

A cDNA sequence coding for feline interferon has been cloned for the first time by screening a cDNA library constructed using Okayama-Berg vector and mRNA derived from the feline cells (LSA-I) induced by TPA (12-o-tetradecanoylphorbor 13-acetate) for the ability of transient expression to produce feline interferon in COS1 monkey cells. The amino acid sequence, deduced from the nucleotide sequence by comparing it with the sequences of other mammalian IFNs, consists of 171 amino acids with 6 cysteins and an N-glycosylation site at the amino acid position 79, and has about 60% homology to human IFN alpha 1. The interferon was partially purified through Blue Sepharose, and its molecular weight was estimated to be 2.4 x 10(4). The antiviral activity was acid stable, and glycosylation was suggested.