核糖体失活蛋白对核糖体拓扑结构的影响

辛纳毒蛋白和克木毒蛋白是本实验室纯化的2种新RIP,它们的作用位点是大鼠肝核糖体285rRNA的A4324.足迹分析表明除 A4324位外,其上、下文的鸟苷酸、腺苷酸也是辛纳毒蛋白和克木毒蛋白的识别位点.辛纳毒蛋白或克木毒蛋白修饰大鼠肝核糖体后,其rRNA的拓扑结构发生了变化,rRNA茎环结构中的双链区相对增多,核糖体的整体拓扑结构也随之变化,80 S核糖体减少,60 S和 40 S亚基增多.以上结果表明“S/R结构域”修饰后所引发的rRNA及核糖体拓扑结构的变化是RIP抑制蛋白质合成的重要机理之一.     

核糖体失活蛋白及核糖体拓扑结构的研究进展

天花粉毒蛋白使核糖体失活的分子机制是它有ＲＮＡＮ－糖苷酶的作用。从樟树种子中纯化的两种新的核糖体失活蛋白（ＲＩＰ）——辛纳毒蛋白和克木毒蛋白也都具有ＲＮＡＮ－糖苷酶和依赖超螺旋结构的核酸内切酶活性。辛纳毒蛋白还有杀虫活性;克木毒蛋白还有超氧化物歧化酶活性。被ＲＮＡＮ－糖苷酶失活的核糖体用硼氢化钠还原或氨基酸加成反应可部分地复活,这表明失活的核糖体ＲＮＡ上产生的一个活泼醛基对其失活起着重要作用。工作中建立了荧光标记在凝胶上测定小分子ＲＮＡ序列和定性测定糖蛋白的两种新方法。     

核糖体失活蛋白与超螺旋DNA相互作用的原子力显微镜直接观察

运用原子力显微镜研究了核糖体失活蛋白 (RIP)与超螺旋DNA相互作用 ,发现这类毒蛋白 (克木毒蛋白和蓖麻毒蛋白A链 ) ,既能与超螺旋形式的DNA结合 ,又能结合在超螺旋DNA分子中未解旋的双链环区 .在与超螺旋DNA结合后 ,引起超螺旋DNA构象变化以利解旋并与双链DNA结合 ,进而将松弛的DNA双链切成缺口或线性形式 .这说明RIP是一种超螺旋DNA结合蛋白 ,并表现出依赖超螺旋的DNA内切酶活性     

眼镜蛇蛇毒的分离及各组分毒性测定

应用羧甲基纤维素盐浓度阶段洗脱柱层析法分离湖南眼镜蛇毒获得15个蛋白峰,其中四个神经毒素峰,产率12%.两神经毒主峰合并对小白鼠皮下注射半数致死量为0.13mg/kg,全毒为1.27mg/kg,广西产克痛宁(眼镜蛇神经毒)为0.35mg/kg。本室制备的蛇神经毒活性较全毒提高近9倍。较广西产克痛宁高1.5倍。聚丙烯酰胺凝胶电泳结果,四个神经毒峰蛋白迁移率分别为0.64,0.70,0.76,0.82。克痛宁为三条神经毒蛋白带,全毒为10条以上蛋白带.     

核糖体失活蛋白的结构功能与分布

核糖体失活蛋白是一类在植物中较广泛存在的毒蛋白。植物核糖体失活蛋白具有RNAN-糖苷酶活力,可作用于核糖体RNA,使核糖体失去蛋白质合成的功能。根据一级结构,核糖体失活蛋白可分为两种类型。Ⅰ型核糖体失活蛋白由一条链组成,分子量在25—30 kDa之间。Ⅱ型核糖体失活蛋白由两条以二硫键相连的链(A、B链)组成,分子量在60 kDa左右。B链可以与细胞表面含半乳糖的受体结合,有助于A链进入细胞,作用于核糖体。目前至少已从9个科31种植物中分离纯化了Ⅰ型RIP。Ⅱ型RIP较少,仅在6科8种植物中发现。除了具有RNA N-糖苷酶活性,还发现一些核糖体失活蛋白可以切割超螺旋双链DNA,产生缺口环状和线状DNA。此外,一种Ⅰ型RIP,克木毒蛋白还具有超氧化物歧化酶活性。     

新丰毒蛋白——一种新的具有活性小A链的核糖体失活蛋白

辛纳毒蛋白是从香樟种子中分离的一种Ⅱ核糖体失活蛋白.最近,从香樟种子中还分离到另一种微型双链核糖体失活蛋白,命名为新丰毒蛋白.还原的新丰毒蛋白表现出与还原的辛纳毒蛋白同样的RNA N-糖苷酶和体外对抑制蛋白质翻译的活力.新丰毒蛋白的B链与辛纳毒蛋白的B链具有同样的分子质量和相同的N端10个氨基酸序列.它的A链N端10个氨基酸序列也与辛纳毒蛋白的A链完全一致,并且C端与辛纳毒蛋白的A链一样具有半胱氨酸,但是它的分子质量却只有辛纳毒蛋白A链的一半.RT-PCR和RNA印迹结果表明体内不存在新丰毒蛋白的mRNA.推测新丰毒蛋白是从辛纳毒蛋白通过蛋白质剪接而产生的,是一种研究蛋白质剪接的好材料.     

新丰毒蛋白——一种新的具有活性小A链的核糖体失活蛋白(英)

辛纳毒蛋白是从香樟种子中分离的一种Ⅱ核糖体失活蛋白.最近,从香樟种子中还分离到另一种微型双链核糖体失活蛋白,命名为新丰毒蛋白.还原的新丰毒蛋白表现出与还原的辛纳毒蛋白同样的RNA N-糖苷酶和体外对抑制蛋白质翻译的活力.新丰毒蛋白的B链与辛纳毒蛋白的B链具有同样的分子质量和相同的N端10个氨基酸序列.它的A链N端10个氨基酸序列也与辛纳毒蛋白的A链完全一致,并且C端与辛纳毒蛋白的A链一样具有半胱氨酸,但是它的分子质量却只有辛纳毒蛋白A链的一半.RT-PCR和RNA印迹结果表明体内不存在新丰毒蛋白的mRNA.推测新丰毒蛋白是从辛纳毒蛋白通过蛋白质剪接而产生的,是一种研究蛋白质剪接的好材料.     

食品上的应用

<正> 853763 通过抗磺胺突变株生产色氨酸[英]/Shiio,L.…∥Agric.Biol.Chem.-1984,48(8).-2073～2080[译自 DBA,1984,3(23),84-11237]将抗5-氟色氨酸和氮丝氨酸的高产率色氨酸生产菌——黄短杆菌 A-100用亚硝基胍进行诱变处理。分离出的突变株是在含1000-2000微克/毫升磺胺的琼脂平板上出现的。突变株225在含13%的葡萄糖作为碳源的培养基中,经72小时培养后产生19克/升的色氨酸,与此相比较亲株 A-100只产生11.3克/升的色氨酸。在含10%的蔗糖培养基上,L-     

色氨酸发酵的研究

<正> L-色氨酸是人和动物体内必需氨基酸之一,在医药、食品和饲料添加方面有着广泛的用途。由于它在动植物蛋白中含量很低,从天然蛋白质中提取来源有限,而化学合成法又代价较高,因此用发酵法来生产L-色氨酸长期以来受到重视。目前主要有直接发酵法,前体发酵法和酶促转化法三种,据报导,1973年Snilo等人用B·subtilis FT~r直接发酵生产L色氨酸,产量达6.1克/升。1973年Nagino等人以及1974、1975年Nagino和NaRaymu等人成功地诱导各种     

植物镉忍耐的分子机理

Cd是植物非必需的微量元素,对植物有很强的毒性.Cd抑制植物细胞生长,抑制氧化磷酸化,引发氧化胁迫,影响光合作用,损伤核仁和影响质膜ATP酶的活力.一些耐Cd植物通过诱导形成螯合肽、金属硫蛋白、植物应激蛋白等抵御Cd毒,也有的耐Cd植物则通过细胞壁固定、液泡分隔、腺体分泌等途径来抵御Cd毒.植物螯合肽合成酶(PCS)相关的一些基因已得到克隆.金属硫蛋白(MT)的克隆基因导入植物,使植物对Cd毒的抗性增加;植物胁迫蛋白可提高植物对Cd毒的抗性,Zn转运蛋白可运转Cd.修饰基因则通过影响主要基因提高植物对Cd的忍耐能力.野生型植物耐Cd毒是多基因控制的,而植物短期的Cd忍耐,则仅受一个或少数基因控制.     

Tryptophan properties in fluorescence and functional stability of plasminogen activator inhibitor 1

Plasminogen activator inhibitor 1 harbors four tryptophan residues at positions 86, 139, 175, and 262. To investigate the contribution of each tryptophan residue to the total fluorescence and to reveal the mutual interactions of the tryptophan residues and interactions with the other amino acids, 15 mutants in which tryptophan residues have been replaced by phenylalanines were constructed, purified, and characterized. Conformational distribution analysis revealed that the tryptophan mutants have a similar conformational distribution pattern as wild-type plasminogen activator inhibitor 1. Mutants in which tryptophan residue 175 was replaced by a phenylalanine displayed an increased functional half-life of the active conformation, whereas the functional half-life of mutants in which tryptophan residue 262 was replaced by a phenylalanine was substantially decreased. Comparative analysis of the fluorescence lifetimes, the extinction coefficients, and the quantum yields of the individual tryptophan residues demonstrates that tryptophan residue 262 gives the highest contribution to the total fluorescence. The other tryptophan residues have a very low quantum yield. In the wild-type protein, the fluorescence of all tryptophan residues is partially quenched as compared to the mutants that contain single tryptophan residues, due to conformational effects. The fluorescence of tryptophan residue 262 is very likely also partially quenched by energy transfer to tryptophan residue 175.     

Role of tryptophan hydroxylase phe313 in determining substrate specificity

The active site residue phenylalanine 313 is conserved in the sequences of all known tryptophan hydroxylases. The tryptophan hydroxylase F313W mutant protein no longer shows a preference for tryptophan over phenylalanine as a substrate, consistent with a role of this residue in substrate specificity. A tryptophan residue occupies the homologous position in tyrosine hydroxylase. The tyrosine hydroxylase W372F mutant enzyme does not show an increased preference for tryptophan over tyrosine or phenylalanine, so that this residue cannot be considered the dominant factor in substrate specificity in this family of enzymes.     

Geranyl modification on the tryptophan residue of ComXRO-E-2 pheromone by a cell-free system

ComX pheromone is an isoprenoidal oligopeptide containing a modified tryptophan residue, which stimulates natural genetic competence in the gram-positive bacterium Bacillus. Since posttranslational prenylation on the tryptophan residue has not been reported except in ComX pheromone, the universality of this modification has not yet been elucidated. In this paper, we established a cell-free system, whereby the tryptophan residue in peptides is modified with a geranyl group by modifying enzyme ComQ. In addition, we investigated enzymatic reaction conditions using an in vitro enzyme reaction system. This is the first report of in vitro geranylation on the tryptophan residue. This system is potentially a useful tool for elucidating the universality of prenylation on the tryptophan residue.     

Identification of the Tryptophan Residue Located at the Saccharide Binding Site of Castor Bean Hemagglutinin

The tryptophan residue present at the saccharide-binding site of castor bean hemagglutinin (CBH) was identified. A peptide containing a modified tryptophan residue was isolated from the tryptic digest of S-car boxy methylated B-chain obtained from an inactive derivative of CBH (2-Oxa-CBH), in which two tryptophan residues/mol were oxidized with Af-bromosuccinimide, by gel filtration on a Sephadex G-50 followed by high performance liquid chromatography. Analytical data for the isolated peptide indicated that the tryptophan residue at position 131 on the B-chain was modified in 2-Oxa-CBH.

From these and earlier results, it is suggested that the tryptophan residue at 131 on each B-chain is closely associated with the saccharide-binding activity of CBH. The specific role of tryptophan residue at 131 in the saccharide-binding site of CBH is also discussed.     

Antisense suppression of proline degradation improves tolerance to freezing and salinity in Arabidopsis thaliana

The location of tryptophan residues in the actin macromolecule was studied on the basis of the known 3D structure. For every tryptophan residue the polarity and packing density of their microenvironments were evaluated. To estimate the accessibility of the tryptophan residues to the solvent molecules it was proposed to analyze the radial dependence of the packing density of atoms in the macromolecule about the geometric center of the indole rings of the tryptophan residues. The proposed analysis revealed that the microenvironment of tryptophan residues Trp-340 and Trp-356 has a very high density. So these residues can be regarded as internal and inaccessible to solvent molecules. Their microenvironment is mainly formed by non-polar groups of protein. Though the packing density of the Trp-86 microenvironment is lower, this tryptophan residue is apparently also inaccessible to solvent molecules, as it is located in the inner region of macromolecule. Tryptophan residue Trp-79 is external and accessible to the solvent. All residues that can affect tryptophan fluorescence were revealed. It was found that in the close vicinity of tryptophan residues Trp-79 and Trp-86 there are a number of sulfur atoms of cysteine and methionine residues that are known to be effective quenchers of tryptophan fluorescence. The most essential is the location of SG atom of Cys-10 near the NE1 atom of the indole ring of tryptophan residue Trp-86. On the basis of microenvironment analysis of these tryptophan residues and the evaluation of energy transfer between them it was concluded that the contribution of tryptophan residues Trp-79 and Trp-86 must be low. Intrinsic fluorescence of actin must be mainly determined by two other tryptophan residues--Trp-340 and Trp-356. It is possible that the unstrained conformation of tryptophan residue Trp-340 and the existence of aromatic rings of tyrosine and phenylalanine and proline residues in the microenvironments of tryptophan residues Trp-340 and Trp-356 are also essential to their blue fluorescence spectrum.     

Correlation between internal motion and emission kinetics of tryptophan residues in proteins

Time-resolved fluorescence anisotropy measurements of tryptophan residues were carried out for 44 proteins. Internal rotational motion with a sub-nanosecond correlation time (0.9 +/- 0.6 ns at 10 degrees C) was seen in a large number of proteins, though its amplitude varied from protein to protein. It was found that tryptophan residues which were almost fixed within a protein had either a long (greater than 4 ns) or short (less than 2 ns) fluorescence lifetime, whereas a residue undergoing a large internal motion had an intermediate lifetime (1.5-3 ns). It is suggested that the emission kinetics of a tryptophan residue is coupled with its internal motion. In particular, an immobile tryptophan residue emitting at long wavelength was characterized by a long lifetime (greater than 4 ns). It appears that a tryptophan residue fixed in a polar region has little chance of being quenched by neighboring groups.     

Synthesis and biological activity of 2-phenylethyl ester analogues of C-terminal heptapeptide of cholecystokinin modified in Trp 30 region.

We have tried to evaluate the significance of the tryptophan side chain residue and of the surrounding peptide bonds in the antagonist activity of cholecystokinin analogues lacking the C-terminal amide function and having a D-tryptophan. In order to perform this study, analogues of the C-terminal heptapeptide of cholecystokinin were synthesized by replacing the C-terminal phenylalanine residue with 2-phenylethyl alcohol and by either replacing the tryptophan residue with an alanine, a norleucine and a phenylalanine residue, or introducing a "reduced peptide bond" in the tryptophan 30 region. Most of these compounds were able to reproduce only part of the response of cholecystokinin in stimulating amylase release from rat pancreatic acini, as was already observed for 2-phenylethyl ester analogues of CCK. These results point out the key role of tryptophan 30 in the biological response of cholecystokinin.     

Role of the tryptophan residue in the vicinity of the catalytic center of exonuclease III family AP endonucleases: AP site recognition mechanism

The mechanisms by which AP endonucleases recognize AP sites have not yet been determined. Based on our previous study with Escherichia coli exonuclease III (ExoIII), the ExoIII family AP endonucleases probably recognize the DNA-pocket formed at an AP site. The indole ring of a conserved tryptophan residue in the vicinity of the catalytic site presumably intercalates into this pocket. To test this hypothesis, we constructed a series of mutants of ExoIII and human APE1. Trp-212 of ExoIII and Trp-280 of APE1 were critical to the AP endonuclease activity and binding to DNA containing an AP site. To confirm the ability of the tryptophan residue to intercalate with the AP site, we examined the interaction between an oligopeptide containing a tryptophan residue and an oligonucleotide containing AP sites, using spectrofluorimetry and surface plasmon resonance (SPR) technology. The tryptophan residue of the oligopeptide specifically intercalated into an AP site of DNA. The tryptophan residue in the vicinity of the catalytic site of the ExoIII family AP endonucleases plays a key role in the recognition of AP sites.     

Nanosecond fluorometry of the single tryptophan in cytochrome P-450e (P450IIB2)

Properties of the single tryptophan residue in rat liver microsomal phenobarbital-inducible cytochrome P-450e (P450IIB2) were studied by the nanosecond time-resolved fluorometry. The tryptophan fluorescence decay time was found to be 3.6 ns and it was not affected by the addition of substrate (perhydrophenanthrene). This result strongly indicates that the tryptophan residue is not a part of the substrate-binding site.     

Significance of the Tryptophan Residue at the Low Affinity Saccharide-binding Site of Ricin E

Chemical modification of tryptophan residues in ricin E was investigated with regard to saccharide-binding. Two out of ten tryptophan residues in ricin E were modified with N- bromosuccinimide at pH 4.5 in the absence of specific saccharide accompanied by a marked decrease in the cytoagglutinating activity. Such a loss of the cytoagglutinating activity was found to be principally due to the oxidation of one tryptophan residue per B-chain. In the presence of lactose, one tryptophan residue/mol was protected from the modification with retention of a fairly high cytoagglutinating activity. However, G a IN Ac did not show such a protective effect. The binding of lactose to ricin E altered the environment of the tryptophan residue at the low affinity binding site of ricin E, leading to a blue shift of the fluorescence spectrum and an UV-difference spectrum with a maximum at 290 nm and a trough at 300 nm. The ability to generate such spectroscopic changes induced by lactose was retained in the derivative in which one tryptophan residue/mol was oxidized in the presence of lactose, but not in the derivative in which two tryptophan residues/mol were oxidized in the absence of lactose. Based on these results, it is suggested that one of the two surface-localized tryptophan residues is responsible for saccharide binding at the low affinity binding site of ricin E, which can bind lactose but lacks the ability to bind GalNAc.