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基因工程９８０１３４人工纤维状蛋白：一篇综述［英］／ＨｅｓｌｏｔＨ．／／Ｂｉｏｃｈｉｍｉｅ．－１９９８，８０（１）．－１９～３１［译自ＤＢＡ，１９９８，１７（１９），９８－０８２７８］从以下方面综述了人工纤维状蛋白（ＡＦＰｓ）：家蚕（Ｂｏｍｂｙｘｍｏ...     

墨兰种子胚的发育和培养初步研究

墨兰种子胚的发育和培养初步研究陈汝民,叶庆生,王小菁,王晓明,郭周义（华南师范大学生物系,广州５１０６３１）关键词墨兰;种子发育;组织培养;原球茎兰属（Ｃｙｍｂｉｄｉｕｍ）植物的种子极小,呈细条状［１］．其中墨兰（Ｃｙｍｂｉｄｉｕｍｓｉｎｅｎｓｅ）种...     

孢堆黑粉菌属三个新组合及中国黑粉菌补遗Ⅷ

本文报道了３个新组合种和３个中国新记录种。新组合是：广州孢堆黑粉菌［Ｓｐｏｒｉｓｏｒｉｕｍ ｃａｎｔｏｎｅｎｓｅ（Ｚｕｎｄｅｌ）Ｌ．Ｇｕｏ］香茅粒孢堆黑粉菌［Ｓｐｏｒｉｓｏｒｉｕｍ ｃｙｍｂｏｐｏｇｏｎｉｓ－ｄｉｓｔａｎｔｉｓ（Ｌｉｎｇ）Ｌ．Ｇｕｏ］和海南孢堆黑粉菌［Ｓｐｏｒｉｓｏｒｉｕｍ ｂａｉｎａｎａｅ（Ｚｕｎｄｅｌ）Ｌ．Ｇｕｏ］。中国新记录种为：中间黑粉菌（Ｕｓｔｉｌａｇｏ ｔａｎａｋａｅ     

豆薯种籽中一种抗真菌蛋白PaAFP的分离纯化和部分特性研究

各类植物由于缺少自身免疫系统的支持,因而必须依赖于其它机制来抵御外来微生物的入侵．其中的一种重要机制就是通过合成体内各类能抑制微生物生长的蛋白质来完成的［１］．已报道从植物中分离出多种不同的抗真菌蛋白．广为研究的是几丁质酶和β－１,３－葡聚糖酶,认为它们在植物对真菌病的抗性中起重要作用［２,３］;核糖体失活蛋白（ＲＩＰｓ）和一类富含半胱氨酸的碱性多肽Ｔｈｉｏｎｉｎｓ也显示有非专一的抗真菌活性［４,５］．但仍有一些蛋白质,体外表现强烈的抗真菌活性,却不属于以上范围［６,７］．本文报道了豆薯种籽中一…     

尖吻蝮蛇出血毒素Ⅲ三维荧光光谱研究

蛇毒中含有多种金属蛋白质,它们具有不同的生物学活性,如抗凝血因子（ＡＣＦ）、糖苷水解酶（ＮＡＤａｓｅ）、纤溶组分（ＦＰ）及出血毒素等,它们的许多生物活性、荧光光谱和结构的性质等方面的研究已见报道［１］．徐洵等［２］从皖南尖吻蝮蛇蛇毒中分离出３种出血毒...     

植物青枯病菌细菌素的产生,性质及其利用

细菌素（Ｂａｃｔｅｒｉｏｃｉｎ）是细菌代谢过程中合成的、对同种或近缘种有特异性抑制作用的杀菌蛋白或多肽物质［１］。大多数植物病原细菌如放射农杆菌（Ａｇｒｏｂａｃｔｅｒｉｕｍ ｒａｄｉｏｂａｃｔｅｒ）、密执安棒形杆菌（Ｃｌａｖｉｂａｃｔｅｒ ｍｉｃｈｉｇａｎｅｓｔｓ）、软腐欧文氏菌（Ｅｒｗｉｎｉａｃａｒｏｔｏｖｏｒａ、 Ｅ． ｃｈｒｙｓａｎｔｈｅｍｉ）、丁香假单胞菌（Ｐｓｅｕｄｏｍｏｎａｓｓｙｒｉｎｇａｅ）、甘蓝黑腐黄单胞菌（Ｘａｎｔｈｏｍｏｎａｓ ｃａｍｐｅｓｔｒｉｓ）等都具有产生细菌素的能力［２］…     

木姜子属生物碱的研究概况(综述)

樟科木姜子属（ＬｉｔｓｅａＬａｍ．）全球约２００种,主要分布于亚洲的热带和亚热带。我国有７２种,在北纬１８°至３４°间均有分布,但主产南方和西南温暖地区,为森林中习见的树木。本属植物的主要用途是提取芳香油（工业上的重要原料）和作为中草药［１］。在我国本属有１７种植物可入药［２］。如药典记载的毕澄茄－山鸡椒（Ｌ．ｃｕｂｅｂａ）的干燥成熟果实,有温中散寒、行气止痛的功效［３］;天目木姜子（Ｌ．ａｕｒｉｃｕｌａｔａ）、木姜子（Ｌ．ｐｕｎｇｅｎｓ）、清香木姜子（Ｌ．ｅｕｏｓｍａ）、潺槁木姜子（Ｌ．ｇｌｕ…     

高蛋白作物四棱豆早熟良种栽培技术及开发利用

四棱豆［Ｐｓｏｐｈｏｃａｒｐｕｓｔｅｔｒａｇｏｎｏｌｏｂｕｓ（Ｌ．）ＤＣ．］是一种地上结荚、地下长薯,根、茎、叶、花、荚、种子均可利用的粮、油、菜、饲、肥、药兼用的高蛋白食用豆类作物。近年来,四棱豆在许多国家较快发展。四棱豆原产潮湿热带地区,属喜温短...     

小葱凝集素的纯化和部分性质研究

小葱凝集素的纯化和部分性质研究林玉满（福建师范大学实验中心生化室,福州３５０００７）凝集素具有众多的生物学性质~［１－４］。自从发现凝集素至今已一百多年,人们已从植物种子或根、茎、叶、韧皮纯化的凝集素有百数十种~［３,５］,但对蔬菜凝集素的研究不多,有...     

微核仁是富含剪接因子SC35的核内小体

许多植物细胞核中存在一些较小的球形或卵圆形的结构,不同作者分别将其称为球体（ｓｐｈｅｒｕｌｅｓ）［１］、核体（ｋａｒｙｏｓｏｍｅ）［２］、核仁附着小体（ｎｕｃｌｅｏｌｕｓａｓｏｃｉａｔｅｄｂｏｄｉｅｓ）［３］、螺旋小体（ｃｏｉｌｅｄｂｏｄｉｅｓ）［４...     

菠菜乙醇酸氧化酶同工酶的亚基组成

我们首次报告 ,菠菜有ＧＯⅠ (ｐＩ≈ 7.4 )、ＧＯⅡ(ｐＩ≈ 9.4 )和ＧＯⅢ (ｐＩ≈ 8.3 ) 3种乙醇酸氧化酶(ＧＯ)同工酶 ;ＧＯⅠ只含 4 0± 2ｋＤ一种亚基 ,而ＧＯⅡ和ＧＯⅢ的亚基组成未被研究 ;3种同工酶之间均有免疫同源性[1-4 ] .水稻也存在 3种ＧＯ同工酶 ,其中ＧＯⅡ (ｐＩ >8.3 )能被乙醇酸所诱导 用柱层析法纯化可获得经ＳＤＳ ＰＡＧＥ后为 4 3± 2ｋＤ单带的水稻ＧＯⅠ[5～ 7] .以上初步解释了前人报告ＧＯ电荷不均一的原因[5] .最近从菠菜分离得到含ＧＯⅡ的蛋白和含ＧＯⅢ的蛋白 ,其ＳＤＳ ＰＡＧＥ分别为 67± 2ｋＤ和 4 0±…     

About three‐fourths of mouse proteins unexpectedly appear at a low position of SDS‐PAGE,often as additional isoforms,questioning whether all protein isoforms have been eliminated in gene‐knockout cells or organisms

Most genes in evolutionarily complex genomes are expressed to multiple protein isoforms, but there is not yet any simple high‐throughput approach to identify these isoforms. Using an oversimplified top‐down LC–MS/MS strategy, we detected, around the 26‐kD position of SDS‐PAGE, proteins produced from 782 genes in a Cdk4?/? mouse embryonic fibroblast cell line. Interestingly, only 213 (27.24%, about one‐fourth) of these 782 genes have their proteins with a theoretical molecular mass (TMM) 10% smaller or larger than 26 kD, that is, between 23 and 29 kD, the range set as allowed variation in SDS‐PAGE. These 213 proteins are considered as the wild type (WT). The remaining three‐fourths includes proteins from 66 (9.44%) genes with a TMM smaller than 23 kD and proteins from 503 (64.32%, nearly two‐thirds) genes with a TMM larger than 29 kD; these proteins are categorized into a larger‐group or a smaller‐group, respectively, for their appearance at a higher or lower position of SDS‐PAGE. For instance, at this 26‐kD position we detected proteins from the Rps27a, Snrpf, Hist1h4a, and Rps25 genes whose proteins' TMM is 8.6, 9.7, 11.4, and 13.7 kD, respectively, and detected proteins from the Plelc1 and Prkdc genes, whose largest isoform is 533.9 and 471.1 kD, respectively. We extrapolate that many of those proteins migrating unexpectedly in SDS‐PAGE may be isoforms besides the WT protein. Moreover, we also detected a Cdk4 protein in this Cdk4?/? cell line, thus wondering whether some of other gene‐knockout cells or organisms show similar incompleteness of the knockout.     

鸡胚骨骼肌组织M-CAT结合因子的初步鉴定

采用偶联ＣＡＴＴＧＣＴ寡核苷酸的ＤＮＡ亲和层析柱从发育１３ｄ鸡胚骨骼肌核抽提物中分离到两种核蛋白．ＳＤＳ－ＰＡＧＥ结果表明,被ＤＮＡ亲和柱滞留的两种核蛋白分子量分别为３０ｋＤ和３２ｋＤ．凝胶阻滞结合竞争分析显示,纯化的核蛋白可与Ｍ－ＣＡＴ共有序列ＣＡＴＴＣＣＴ特异结合．Ｓｏｕｔｈｗｅｓｔｅｒｎ印迹技术确定仅３０ｋＤ分子可直接识别、结合ＣＡＴＴＣＣＴ元件,但３２ｋＤ分子却不能．结果提示,３０ｋＤ分子为依赖ＤＮＡ的Ｍ－ＣＡＴ结合因子,３２ｋＤ分子属性有待进一步研究证实     

p16抑癌基因定点突变及其在大肠杆菌中的表达与纯化

为了研究错义突变对ｐ１６功能的影响,应用ＰＣＲ体外定点突变方法对ｐ１６ｃＤＮＡ进行体外定点突变,并将野生型和突变型ｐ１６ｃＤＮＡ克隆于ｐＧＥＸ－５Ｔ载体,在大肠杆菌中经ＩＰＴＧ诱导表达,Ｗｅｓｔｅｒｎ印迹鉴定确证表达．而后用谷胱甘肽－Ｓｅｐｈａｒｏｓｅ４Ｂ亲和层析纯化野生型和突变型ｐ１６融合蛋白．得到了第４８位密码子ＣＣＧ（Ｐｒｏ）→ＣＴＧ（Ｌｅｕ）突变的ｐ１６－Ｐ４８突变体,并在大肠杆菌中表达了４２ｋＤ的ＧＳＴ－ｐ１６和ＧＳＴ－ｐ１６Ｐ４８Ｌ融合蛋白．最后经纯化得到了野生和Ｐ４８Ｌ突变的ｐ１６融合蛋白     

Characterization of a 24 kD parasitism-specific hemolymph protein from pharate pupae of the caribbean fruit fly,Anastrepha suspensa

A parasitism-specific protein was originally identified in the hemolymph of the Caribbean fruit fly Anastrepha suspensa parasitized by the braconid wasp Diachasmimorpha (Biosteres) longicaudata using single-dimensional (1-D) sodium dodecyl sulfate (SDS) PAGE. We now show that the protein is comprised of two closely migrating species both of which are glycoproteins of ≈? 24,000 Daltons (24 kD). The proteins were poorly resolved from whole hemolymph by 1-D SDS PAGE, but were well resolved by two-dimensional (2-D) PAGE and isoelectric focusing. They have pl's of ≈? 6.3 and 6.7 and contain Man residues, based on their affinity for concanavalin A (Con A). The presence of GlcNAc, NeuAc, and GalNAc residues in both proteins was implicated by their binding to wheat germ agglutinin (WGA). The proteins bound WGA more intensely following mannosidase treatment which eliminated their affinity to Con A and further implicated the presence of internal GlcNAc residues. However, binding of the proteins to WGA in the presence of competing GlcNAc (1 M) was reduced but not eliminated and suggested that in addition to GlcNAc, other WGA-binding sugar moieties, possibly NeuAc, a Sia, were present. To evaluate the presence of NeuAc, we treated the hemolymph with Vibrio cholerae neuraminidase which specifically cleaves terminal Sia. Samples of the neuraminidase-digested proteins were evaluated by WGA binding and Western blotting with the use of an anti-24 kD rabbit polyclonal serum to determine whether desialation eliminated the proteins' affinity to WGA or their immunoreactivity. Our results show that partial digestion of the 24 kD proteins with Vibrio cholerae neuraminidase resulted in two immunoreactive bands in Western blots of 1-D gels but only one of these, the upper undigested 24 kD band, bound WGA. This confirmed the presence of Sia residues in the proteins and demonstrated that desialation increased their relative electrophoretic mobilities. © 1994 Wiley-Liss, Inc.     

菜心和水稻绿叶中不同等电点的乙醇酸氧化酶

The proteins with glycolate oxidase activity from B.parachinensis Bailey and rice( Oryza sativa )green leaves were prepared respectively.From the second protein peak on DEAE\|Cellulose column,two glycolate oxidases,expressed as B.parachinensis Bailey GO Ⅲ(specific activity natove 13 2 U·mg -1 ·min -1 )and rice GOⅢ(specific activity 8 8 U·mg -1 ·min -1 ),could not migrate anywhere in 4%～20% native\|PAGE under a pH8.3 buffer system.GOⅢ's p I was about pH8.3. The protein containing B.parachinensis Bailey GOⅢ showed 67±2,43±2,and 38±2 kD in SDS PAGE,band 43±2 kD was the subunit of B.parachinensis Bailey GOⅢ.From the two proteins above,another group of glycolate oxidases,expressed as B.parachinensis Beiley GOⅠ(specific activity 5 U·mg -1 ·min -1 )and rice GOⅠ(specific activity 1 2 U·mg -1 ·min -1 ),showed only one 43±2 kD band in SDS\|PAGE,and was purified on the Sepharose\|6B column which migrated towards anode in the same native\|PAGE showing the M r about 420 kD,or 460 kD and 260 kD respectively.GOⅠ's p I was smaller than pH8.3.Antibody against B.parachinensis Bailey GOⅠ was prepared and its efficacy was about 1/1600 in ELISA.By native\|PAGE,Western blot and rocket immunoelectrophoresis,the third group of glycolate oxidases,expressed as B.parachinensis Bailey GOⅡ and rice G0Ⅱ,were confirmed in crude protein of green leaves and migrated towards cathode under the same native\|PAGE,so GOⅡ's p I was higher than pH8.3.The M r of B.parachinensis Bailey GOⅡ was about 669 kD determined by native\|PAGE Western blot.Rice GOⅠ,rice GOⅢ and rice GOⅡ showed different quantitation under different physiological conditions.Rice GOⅡ could be induced by glycolate.     

兔阑尾中一种新的21kD的钙结合蛋白的纯化与鉴定

纯化与鉴定了Ｂ淋巴细胞中一种新的分子量为２１ｋＤ的钙结合蛋白（ＣａＢＰ２１）。兔阑尾淋巴细胞匀浆经热变性,Ｐｈｅｎｙｌ－Ｓｅｐｈａｒｏｓｅ与ＤＥＡＥ－Ｓｅｐｈａｒｏｓｅ柱层析,自每１ｋｇ细胞沉积物中获得ＳＤＳ－ＰＡＧＥ均一的ＣａＢＰ２１５．３ｍｇ。ＨＣｌ水解后的酸性氨基酸（Ａｓｐ＋Ｇｌｕ）含量为２６％。如同大多数钙结合蛋白一样,Ｎ末端封闭阻止其进行Ｅｄｍａｎ降解。ＣａＢＰ２１中疏水性氨基酸（计Ｇｌｙ,不计Ｔｒｐ）约占４６％,碱性氨基酸１０％,酸性氨基酸与极性氨基酸约４４％。ＣａＢＰ２１有较高的Ｓｅｒ、Ｔｙｒ含量。肽谱分析等确证ＣａＢＰ２１为２个相同或相似亚基二聚体。以ＡｒｓｅｎａｚｏⅢ作Ｃａ２＋结合分析表明每分子ＣａＢＰ２１可结合４分子Ｃａ２＋,对Ｃａ２＋的结合常数约为１０－５ｍｏｌ／Ｌ。各种性质表明ＣａＢＰ２１是一种不同于其他已知钙结合蛋白的新钙结合蛋白。     

荔枝胚败育过程中内源激素与蛋白质含量的变化

连续3年(1999-2001年)对典型的荔枝焦核品种桂味、糯米糍和大核品种黑叶、怀枝花后10-40d的幼胚和胚乳内源激素、多酚含量及蛋白质动态变化进行研究。结果表明,焦核品种幼胚及胚乳中的IAA、GAs和ABA含量低于大核品种;多酚类物质含量在胚中低于大核品种,胚乳中则高于大核品种;胚和胚乳中的蛋白质含量均低于大核品种。蛋白质电泳结果显示,22．5、28．5和45kD这3类蛋白质在怀枝和黑叶的胚蛋白质代谢过程中表现出较高的稳定性,桂味和糯米糍胚蛋白质中的28．5kD蛋白质也有相似的特性。     

人肝细胞生长因子(hdHGF)基因在毕赤酵母中的分泌表达

研究了hdHGF基因在毕赤酵母中的表达 .以人胎盘mRNA为模板 ,经逆转录、重叠PCR获得hdHGF全长和成熟基因片段 .将该基因片段克隆到pPIC9载体上 ,将重组表达质粒转化巴斯德毕赤酵母 (Pichiapastoris)GS115,筛选mut+ 表型 ,经甲醇诱导可实现rhdHGF的分泌表达 .经摇瓶培养筛选出 4株表达水平较高的酵母工程菌株 ,SDS PAGE分析和Western印迹试验表明 ,产物分子量约为80kD ,5L发酵罐高密度培养已使生物量达 13 5g L(干重 ) ,发酵液上清总蛋白量为 8 0g L ,电泳结果表明rhdHGF表达水平为总蛋白的 12 3 % .     

丙型肝炎病毒Core与NS3基因的不同融合方式及其表达

丙型肝炎病毒(简称ＨＣＶ)是危害人类健康的传染性疾病,预防该病的传播主要借助于ＨＣＶ血清学诊断来筛选献血员和检测临床标本。从国内外已分离到的ＨＣＶ株得知,ＨＣＶ核心蛋白(Ｃｏｒｅ)和非结构蛋白ＮＳ3含有较强的优势抗原表位,其相应的抗体出现早,阳性率高,已成为目前第二、第三代ＨＣＶ免疫诊断试剂的重要成份[1,2]。通常Ｃｏｒｅ蛋白和ＮＳ3蛋白分别用基因工程方法表达,然后作为固定化抗原,检测人体内ＨＣＶ的抗体。我们对Ｃｏｒｅ和ＮＳ3的两种不同组合方式及其表达的研究,对于发展新的ＨＣＶ诊断试剂很有帮助,现将结果报道如下。1…