小立碗藓扩展蛋白基因家族的鉴定与生物信息学分析

扩展蛋白(Expansins,EXP)是一类基因家族,几乎参与了植物发育的全过程,从种子萌发到果实成熟都有扩展蛋白的参与。该研究利用生物信息学的方法对小立碗藓(Physcomitrella patens) Expansin基因家族成员进行鉴定,分析了其基因结构、染色体定位以及系统发生关系。结果表明:小立碗藓基因组中含有Expansin A(EXPA) 32个、Expansin-like A(EXLA) 6个,并未发现Expansin-like B(EXLB)及Expansin B(EXPB)。扩展蛋白氨基酸序列长度在228～290 aa之间,编码蛋白质具有两个保守的结构域Pollen_allerg_1和DPBB_1。蛋白质亚细胞定位预测结果表明:运用CELLO在线工具预测发现小立碗藓中约4/5的EXP家族基因定位于细胞外;而Euk-mPLoc预测结果则显示小立碗藓EXP基因家族成员全定位于细胞外。基因结构分析表明,小立碗藓中约68%Expansin基因有含有1～3个内含子。以上结果可为深入研究小立碗藓扩展蛋白基因的分子进化与生物学功能奠定基础。     

毛竹谷胱甘肽过氧化物酶基因分子特征及其表达模式分析

利用生物信息学以及分子生物学方法对毛竹(Phyllostachys edulis (Carriere) J. Houzeau)谷胱甘肽过氧化物酶基因(GPX)的分子特征以及表达模式进行分析。结果显示,在毛竹中共鉴定出9个GPX家族成员基因(PeGPX1-PeGPX9),均具有6个外显子以及5个内含子,PeGPXs编码蛋白的长度为168~235 aa,相对分子量在18.41~25.54 kD,等电点范围为5.88~9.48。亚细胞定位预测结果发现,除PeGPX5定位在线粒体上,其他PeGPXs都定位在叶绿体上。在PeGPXs启动子中含有多种与胁迫和激素相关的顺式作用元件。qRT-PCR分析结果表明,强光、低温、GA₃、NAA和MeJA处理均可引起毛竹叶片中PeGPXs表达量发生明显变化。     

丹参谷胱甘肽过氧化物酶的生物信息学分析

谷胱甘肽过氧化物酶(glutathione peroxidase, GPX)是动植物体内一种重要的抗氧化酶,它能够清除机体逆境胁迫而产生的过氧化氢和脂质过氧化物,使机体进行正常生长发育,因此解析丹参GPX的氨基酸序列,并与其它植物进行比较,为丹参GPX基因的后续研究提供重要参考。采用生物信息学的方法,在丹参基因组库中找到8个GPX基因,并对其进行生物信息学分析。8个GPX基因有不同的等电点和相对分子量,而二级结构存在相似特征;序列比对与系统发生分析表明,8个基因都具有3个保守结构域以及3个保守的催化残基;除Sm GPX4、At GPX4和Zm GPX02,Sm GPX8与At GPX8处于系统进化树的同一分支外,其它基因与玉米和拟南芥GPX基因的亲缘关系较远;Sm GPX1-2、Sm GPX6-1、Sm GPX6-2、Sm GPX8主要在叶片中表达,而Sm GPX1-1主要在花中表达,具有组织特异性。本研究为进一步了解丹参谷胱甘肽过氧化物酶的基本功能奠定了基础,为开展植物抵御氧化胁迫研究提供了理论依据。     

水稻谷胱甘肽过氧化物酶基因OsGPX3 和OsGPX4的分子特性研究

植物谷胱甘肽过氧化物酶(glutathione peroxidase,GPX)是清除体内活性氧的一种关键酶,在植物抗逆反应中发挥重要作用.本研究从水稻中克隆到2个GPX基因,分别为OsGPX3和OsGPX4.OsGPX3和OsGPX4分别编码238和234个氨基酸组成的蛋白质,预测分子量分别是25.84 kD和25.07 kD.两个基因都包含5个内含子,但是两个基因所对应的内含子长度具有较大变异.组织表达谱分析发现这2个基因在根、茎、叶和叶鞘中均表达,是组成型表达基因.在大肠杆菌中表达并纯化了这2个基因的重组蛋白,酶活性分析显示OsGPX3和OsGPX4蛋白对底物H₂O₂、tBOOH和COOH具有较高活性,但是OsGPX3对3种底物的活性均高于OsGPX4,蛋白质酶活性的差异预示着这2个基因可能存在功能上的分化.     

小立碗藓WRKY基因家族生物信息学分析

WRKY作为最先在植物中发现的转录因子,在植物生长发育等过程中发挥重要作用。为了更好地研究小立碗藓WRKY蛋白的结构与功能,该文以Pfam数据库中WRKY基因家族数据(登录号为PF03106)为材料,分析了小立碗藓(Physcomitrella patens)WRKY基因家族成员的理化性质、蛋白质的二级结构预测、染色体定位、内外显子分布及系统进化关系。结果表明:(1)小立碗藓WRKY基因家族成员共有38个基因,根据WRKY保守结构域个数和锌指结构类型分成Ⅰ、Ⅱ两大类,不含第Ⅲ类(锌指结构为C2HC型),其中部分基因WRKY保守结构域发生变异。(2)WRKY蛋白氨基酸长度在216~775 aa之间、相对分子质量在24.5~82.8 kDa之间,亚细胞定位显示WRKY家族成员蛋白质定位于细胞核中。(3)WRKY蛋白的二级结构以α-螺旋、延伸链、β-转角、无规卷曲四种构成元件构成,除PpWRKY11(α-螺旋为主)外,其余无规卷曲占比高达70%。(4)与拟南芥的系统进化关系表明,植物在进化过程中WRKY家族成员的数目与进化方式发生改变,WRKY基因家族成员外显子的个数为3~7个。(5)小立碗藓WRKY基因家族成员无规则分散于21条染色体上,并未形成基因簇。该研究通过分析WRKY基因家族的基本结构与性质,能为后续深入研究WRKY转录因子的功能奠定基础。     

盐芥谷胱甘肽过氧化物酶基因（ThGPX6）的克隆及表达分析

谷胱甘肽过氧化物酶在植物响应盐胁迫中具有重要作用。依据盐芥EST序列进行RACE实验,获得1个新的谷胱甘肽过氧化物酶基因,命名为ThGPX6(GenBank注册号为FJ357244)。该基因的cDNA全长892 bp,包含1个长为702bp的开放读码框,编码234个氨基酸。生物信息学分析表明,该蛋白具有植物GPX的典型结构,即GPX催化活性区(NVASKCGLT)和标志性基序(ILAFPCNQF),以及PHGPX特有序列(KWNF(S/T)KFL)。实时荧光定量PCR分析结果表明,ThGPX6在盐芥叶片和根中表达,其表达受NaCl诱导,显示ThGPX6在植物高盐响应中发挥作用。亚细胞定位结果表明,ThGPX6存在于线粒体和内体中的可能性最大,预示着ThGPX6在清除ROS过程中起着重要作用。     

小立碗藓PpAGO7基因的克隆及表达分析

该研究采用同源克隆的方法获得了小立碗藓AGO7蛋白编码基因PpAGO7,对PpAGO7基因序列特征进行生物信息学分析,并利用Real-time PCR方法分析PpAGO7基因的时空表达模式,为揭示小立碗藓中PpAGO7基因的生物学功能提供依据。结果表明:PpAGO7基因的全长cNDA为3 583bp,其中开放阅读框3 363bp,编码1 120个氨基酸,分子量123.38kD,等电点9.26,含有AGO蛋白典型的PAZ和PIWI结构域;PpAGO7基因在小立碗藓整个生活周期都有表达,且在茎叶体生长时期表达水平较高,但在原丝体时期表达水平较低。研究结果推测PpAGO7基因可能在茎叶体拟叶的生长发育过程中起作用。     

江南卷柏Phi类谷胱甘肽S-转移酶的分子特性

谷胱甘肽S-转移酶(Glutathione S-transferase,GST)在帮助植物抵抗各种胁迫中发挥重要作用。该研究从江南卷柏Selaginella moellendorffii中克隆到两个Phi类GST基因,分别命名为Sm GSTF1和Sm GSTF2,两个基因均编码215个氨基酸残基的蛋白质。表达模式分析发现,这两个基因在江南卷柏根、茎和叶中均有表达。将这两个基因在大肠杆菌中诱导表达重组蛋白并纯化,酶学性质分析表明Sm GSTF1和Sm GSTF2对CDNB、NBD-Cl和NBC等3种底物都有活性。Sm GSTF1对Fluorodifen和Cum-OOH也有活性,而Sm GSTF2对它们没有活性。酶动力学分析表明Sm GSTF1和Sm GSTF2对GSH有较高的亲和力,而对CDNB的亲和力都相对较低。在不同p H及温度条件下对Sm GSTF1和Sm GSTF2重组蛋白进行活性测定,发现这两个蛋白在p H 7-8.5,45-55℃温度范围内有较高的催化活性。研究推测,Sm GSTF1和Sm GSTF2可能在江南卷柏的抗逆生理过程中有重要的作用。     

罗非鱼微囊藻毒素去毒相关基因克隆与活体表达研究

可溶性谷胱甘肽S-转移酶(Soluble glutathione S-transferase,sGST)催化微囊藻毒素(Microcystins,MCs)与还原型谷胱甘肽(GSH)的加合去毒代谢过程,谷胱甘肽过氧化物酶(Glutathione peroxidase,GPX)为sGST的去毒反应提供GSH,解偶联蛋白2(Uncoupling protein 2,UCP2)则可抑制微囊藻毒素诱发活性氧导致的肝细胞凋亡。本研究从罗非鱼肝脏通过简并引物克隆sGST、GPX与UCP2基因cDNA核心序列,并应用5’RACE和3’RACE技术分别扩增罗非鱼肝脏sGST基因cDNA序列5’末端和3’末端序列而获得其cDNA全序列。罗非鱼肝脏sGST基因cDNA全序列长861 bp,其中5’非翻译区(5-’UTR)为25 bp,3’非翻译区(3-’UTR)为167 bp,开放阅读框(ORF)为669 bp,编码222个氨基酸,包含脊椎动物完整sGST的2个功能域:N-末端功能域(GSH结合位点)和C-末端功能域(底物结合位点)。罗非鱼sGST与真鲷、条石鲷(Oplegnathus fasciatus)、斑马鱼同源性较高,达到64.3%—78.5%,而与人、大鼠、小鼠、牛、猪、鸡差异较大,氨基酸同源性为48.2%—55.9%。罗非鱼肝脏GPX、UCP2基因cDNA核心序列长280 bp、776 bp,分别编码92、258个氨基酸。罗非鱼GPX与条石鲷、虹鳟、斑马鱼、人、大鼠、小鼠、牛、猪GPX同源性均较高,达到69.6%—85.9%。罗非鱼UCP2与真鲷、斑马鱼、鲤鱼、欧洲白鲑(Leuciscus cephalus)、草鱼、人、大鼠、小鼠UCP2同源性更高,达到71.8%—93.8%。通过对罗非鱼(5—8 g)活体腹腔注射亚致死量MC-LR(50μg/kg bwt),发现微囊藻毒素对罗非鱼肝脏sGST基因表达有显著的诱导作用(p<0.05),注射微囊藻毒素24h后sGST基因mRNA表达水平上调80%。注射微囊藻毒素24h后,虽然罗非鱼肝脏GPX与UCP2基因mRNA表达水平亦出现明显的升高趋势,但两者均未出现显著性的变化(p>0.05)。本研究从基因表达调控的角度证实,罗非鱼肝脏sGST在微囊藻毒素去毒过程中可能发挥关键作用,同时也说明罗非鱼肝脏GPX、UCP2基因可能在微囊藻去毒过程中发挥协同作用。     

草鱼胞浆谷胱甘肽过氧化物酶cDNA全长的克隆与分析

谷胱甘肽过氧化物酶(glutathione peroxidases,GPXs,EC1.11.19)是生物体内抗氧化防御系统的重要组成部分。本文从草鱼(Ctenopharyngodon idellus)克隆到胞浆谷胱甘肽过氧化物酶基因(GPX1)cDNA全长序列。该序列全长890bp(GenBank accession No.EU828796),包括完全开放阅读框(ORF)576bp、5'非编码区(5'-UTR)17bp和3'-UTR297bp。其ORF编码191个氨基酸残基,包含一个由"UGA"(通常为终止密码子)编码的硒代半胱氨酸(selenocysteine,Sec40)残基,并与另2个残基(Glu75和Trp153)构成酶活性中心。同时,草鱼GPX1cDNA的3'-UTR中具有保守的硒代半胱氨酸插入序列(selenocysteine insertion sequence,SECIS)元件。氨基酸序列相似性比较显示,草鱼GPX1cDNA的推测氨基酸序列(GenBank accession No.ACF39780)与斑马鱼GPX1(GenBank accession No.NP_001007282)的相似性为95.8%,与鳗鲡GPX1(GenBank acces-sion No.ACN78878)的为84.8%,与哺乳类的为59%~72%。采用实时荧光定量PCR(Q-PCR)检测草鱼GPX1的组织表达特征。结果表明,草鱼GPX1的mRNA在所检测的11种组织器官中均有表达,其中在肝、鳃和肾表达水平较高,在红肌、脂肪和肠道中表达水平较低。本研究结果将有助于进一步探讨鱼类GPX1基因的结构与功能,并为研究其抗氧化分子机理奠定基础。     

Molecular and Catalytic Properties of Glutathione Peroxidase Family Proteins from Pinus tabulaeformis

Glutathione peroxidase (GPX) is one of the key enzymes that protect cells against oxidative damage caused by reactive oxygen species. Previous studies of plant GPXs focused mainly on angiosperms. In contrast, little information is available on the molecular characteristics of this gene family in gymnosperms. In this study, four GPX genes (PtaGPX1, 2, 3, and 4) were cloned from the gymnosperm Pinus tabulaeformis, which showed high protein sequence identity and similar expression patterns in various tissues. The four Pinus GPX proteins were expressed in Escherichia coli, and the purified proteins used thioredoxin, but not glutathione, as an electron donor. The four Pinus GPXs showed different enzymatic activities and kinetic characteristics, suggesting functional divergence. Two conserved Cys residues (corresponding to Cys44 and Cys92 of PtaGPX3) were identified in all plant GPXs, and their functions were assessed using site-directed mutagenesis. Cys44 and Cys92 of PtaGPX3 could form an intramolecular disulfide bond under oxidizing conditions. These two residues were critical components of active sites and contributed to catalytic activity. This study provides novel insights into the functional divergence and catalytic properties of the GPX family in gymnosperms.     

Roles of the N-terminal domain and remote substrate binding subsites in activity of the debranching barley limit dextrinase

Barley limit dextrinase (HvLD) of glycoside hydrolase family 13 is the sole enzyme hydrolysing α-1,6-glucosidic linkages from starch in the germinating seed. Surprisingly, HvLD shows 150- and 7-fold higher activity towards pullulan and β-limit dextrin, respectively, than amylopectin. This is investigated by mutational analysis of residues in the N-terminal CBM-21-like domain (Ser14Arg, His108Arg, Ser14Arg/His108Arg) and at the outer subsites +2 (Phe553Gly) and +3 (Phe620Ala, Asp621Ala, Phe620Ala/Asp621Ala) of the active site. The Ser14 and His108 mutants mimic natural LD variants from sorghum and rice with elevated enzymatic activity. Although situated about 40 Å from the active site, the single mutants had 15–40% catalytic efficiency compared to wild type for the three polysaccharides and the double mutant retained 27% activity for β-limit dextrin and 64% for pullulan and amylopectin. These three mutants hydrolysed 4,6-O-benzylidene-4-nitrophenyl-6³-α-d-maltotriosyl-maltotriose (BPNPG3G3) with 51–109% of wild-type activity. The results highlight that the N-terminal CBM21-like domain plays a role in activity. Phe553 and the highly conserved Trp512 sandwich a substrate main chain glucosyl residue at subsite +2 of the active site, while substrate contacts of Phe620 and Asp621 at subsite +3 are less prominent. Phe553Gly showed 47% and 25% activity on pullulan and BPNPG3G3, respectively having a main role at subsite +2. By contrast at subsite +3, Asp621Ala increased activity on pullulan by 2.4-fold, while Phe620Ala/Asp621Ala retained only 7% activity on pullulan albeit showed 25% activity towards BPNPG3G3. This outcome supports that the outer substrate binding area harbours preference determinants for the branched substrates amylopectin and β-limit dextrin.     

Decolourisation of anthraquinone-and anthracene-type dyes by versatile peroxidases from bjerkandera fumosa and pleurotus ostreatus D1

The catalytic properties of a versatile peroxidase from Pleurotus ostreatus D1 (Jacquin) P. Kummer were studied in comparison with that of a typical versatile peroxidase from Bjerkandera fumosa 137 (Per.:Fr) Karst. Decolourisation activities of both enzymes towards a wide range of dyes containing condensed aromatic rings (anthraquinone- and anthracene-type) were found. The anthraquinone dyes were decolourised rapidly by both tested peroxidases. The presence of polymerisation reaction products of Acid Blue 62, Basic Blue 22 and Reactive Blue 4 oxidation, and breakdown of aromatic rings of Alizarin Red were observed. The main catalytic constants (KM and Vmax) of the decolourisation reactions of anthraquinone dyes were calculated. In the case of Alizarin Red, inhibition of the activity of versatile peroxidase from P. ostreatus D1 by an excess of the substrate was observed. Independence from Mn²⁺ ions of the catalytic activity of versatile peroxidase from P. ostreatus D1 towards different substrates was revealed. Finally, differences in the catalytic activity towards anthracene-type dyes and monoaromatic substrates of both peroxidases were found.     

Arg<Superscript>235</Superscript> is an essential catalytic residue of <Emphasis Type="Italic">Bacillus pumilus</Emphasis> DKS1 pectate lyase to degum ramie fibre

After 24 h of incubation with only purified pectate lyase isolated from Bacillus pumilus DKS1 (EF467045), the weight loss of the ramie fibre was found to be 25%. To know the catalytic residue of pectate lyase the pel gene encoding a pectate lyase from the strain Bacillus pumilus DKS1 was cloned in E. coli XL1Blue and expressed in E. coli BL21 (DE3) pLysS. The pel gene was sequenced and showed 1032 bp length. After purification using CM-Sepharose the enzyme showed molecular weight of 35 kDa and maximal enzymatic activity was observed at 60°C and a pH range of 8.5–9.0. Both Ca²⁺ and Mn²⁺ ions were required for activity on Na-pectate salt substrates, while the enzyme was strongly inhibited by Zn²⁺ and EDTA. The deduced nucleotide sequence of the DKS1 pectate lyase (EU652988) showed 90% homology to pectate lyases from Bacillus pumilus SAFR-032 (CP000813). The 3D structure as well as the catalytic residues was predicted using EasyPred software and Catalytic Site Atlas (CSA), respectively. Site directed mutagenesis confirmed that arginine is an essential catalytic residue of DKS1 pectate lyase.     

The importance of starch and sucrose digestion in nutritive biology of synanthropic acaridid mites: α‐Amylases and α‐glucosidases are suitable targets for inhibitor‐based strategies of mite control

The adaptation of nine species of mites that infest stored products for starch utilization was tested by (1) enzymatic analysis using feces and whole mite extracts, (2) biotests, and (3) inhibition experiments. Acarus siro, Aleuroglyphus ovatus, and Tyroborus lini were associated with the starch‐type substrates and maltose, with higher enzymatic activities observed in whole mite extracts. Lepidoglyphus destructor was associated with the same substrates but had higher activities in feces. Dermatophagoides farinae, Chortoglyphus arcuatus, and Caloglyphus redickorzevi were associated with sucrose. Tyrophagus putrescentiae and Carpoglyphus lactis had low or intermediate enzymatic activity on the tested substrates. Biotests on starch additive diets showed accelerated growth of species associated with the starch‐type substrates. The inhibitor acarbose suppressed starch hydrolysis and growth of the mites. We suggest that the species with higher starch hydrolytic activity in feces were more tolerant to acarbose, and α‐amylase and α‐glucosidase of synanthropic mites are suitable targets for inhibitor‐based strategies of mite control. © 2009 Wiley Periodicals, Inc.     

Isolation and properties of fungal β-glucosidases

Using chromatography on different matrixes, three β-glucosidases (120, 116, and 70 kDa) were isolated from enzymatic complexes of the mycelial fungi Aspergillus japonicus, Penicillium verruculosum, and Trichoderma reesei, respectively. The enzymes were identified by MALDI-TOF mass-spectrometry. Substrate specificity, kinetic parameters for hydrolysis of specific substrates, ability to catalyze the transglucosidation reaction, dependence of the enzymatic activity on pH and temperature, stability of the enzymes at different temperatures, adsorption ability on insoluble cellulose, and the influence of glucose on catalytic properties of the enzymes were investigated. According to the substrate specificity, the enzymes were shown to belong to two groups: i) β-glucosidase of A. japonicus exhibiting high specific activity to the low molecular weight substrates cellobiose and pNPG (the specific activity towards cellobiose was higher than towards pNPG) and low activity towards polysaccharide substrates (β-glucan from barley and laminarin); ii) β-glucosidases from P. verruculosum and T. reesei exhibiting relatively high activity to polysaccharide substrates and lower activity to low molecular weight substrates (activity to cellobiose was lower than to pNPG).     

Molecular cloning and purification of an endochitinase from Serratia marcescens (Nima)

An endochitinase gene from the Serratia marcescens Nima strain (chiA Nima) was cloned, sequenced, and expressed in Escherichia coli DH5αF′, and the recombinant protein (ChiA Nima) was purified by hydrophobic interaction chromatography. chiA Nima contains an open reading frame (ORF) that encodes an endochitinase with a deduced molecular weight and an isoelectric point of 61 kDa and 6.84, respectively. A sequence at the 5′-end was identified as a signal peptide, recognized by Gram-negative bacteria transport mechanism. Comparison of ChiA Nima with other chitinases revealed a modular structure formed by the catalytic domain and a putative chitin-binding domain. The purified chitinase was able to hydrolyze both trimeric and tetrameric fluorogenic substrates, but not a chitobiose analog substrate. ChiA Nima showed high enzymatic activity within a broad pH range (pH 4.0–10.0), with a peak activity at pH 5.5. The optimal temperature for enzymatic activity was detected at 55°C.     

The cold-active Lip1 lipase from the Antarctic bacterium Pseudoalteromonas haloplanktis TAC125 is a member of a new bacterial lipolytic enzyme family

The genome of the Antarctic bacterium Pseudoalteromonas haloplanktis TAC125 was searched for the presence of genes encoding ester-hydrolysing enzymes. Amongst the others, the gene PSHAa0051 coding for a putative secreted esterase/lipase was selected. The psychrophilic gene was cloned, functionally over-expressed in P. haloplanktis TAC125, and the recombinant product (after named PhTAC125 Lip1) was purified. PhTAC125 Lip1 was found to be associated to the outer membrane and exhibited higher enzymatic activity towards synthetic substrates with long acyl chains. A structural model was constructed using the structure of carboxylesterase Est30 from Geobacillus stearothermophilus as template. The model covered the central part of the protein with the exceptions of PhTAC125 Lip1 N- and C-terminal regions, where the psychrophilic protein displays extra-domains. The constructed model showed a typical α/β-hydrolase fold, and confirmed the presence of a canonical catalytic triad consisting of Ser, Asp and His. The sequence analysis showed that PhTAC125 Lip1 is distantly related to other lipolytic enzymes, but closely related to other putative psychrophilic esterases/lipases. The aligned proteins share common features, such as: (1) a conserved new active-site pentapeptide motif (LGG(F/L/Y)STG); (2) the likely extra-cytoplasmic localization, (3) the absence of a typical calcium-binding pocket, and (4) the absence of a canonical lid. These observations strongly suggest that aligned proteins constitute a novel lipase family, typical of psychrophilic marine γ-proteobacteria, and PhTAC125 Lip1 could be considered the first characterised member of this family. Electronic supplementary material The online version of this article (doi:) contains supplementary material, which is available to authorized users. D. de Pascale and A. M. Cusano equally contributed to the work.     

拟南芥谷胱甘肽S-转移酶Zeta类进化酶的获得及其特性分析

拟南芥谷胱甘肽S-转移酶Zeta类(AtGSTZ)是一种与细胞代谢和环境净化密切相关的多功能酶.应用易错PCR和多轮DNA洗牌技术构建了AtGSTZ随机突变文库;再利用pH指示剂颜色改变法对突变文库进行筛选,获得了9个二氯乙酸脱氯活性提高的突变子.其中,NN23含25个氨基酸突变,比活力提高120%,NN20含24个氨基酸突变,比活力提高102%,EC1含2个氨基酸突变,比活力提高47%,其他6个为单点突变,比活力分别提高9%～60%.酶学分析显示,所有进化酶对底物二氯乙酸的催化效率和对谷胱甘肽的亲和力以及个别进化酶的复性能力都得到不同程度的提高,但热稳定性均没有明显改善.同时,对一系列与AtGSTZ空间折叠及催化活性相关位点进行了讨论.     

Myrosinases from root and leaves of Arabidopsis thaliana have different catalytic properties

Myrosinases (EC 3.2.1.147) are β-thioglucoside glucosidases present in Brassicaceae plants. These enzymes serve to protect plants against pathogens and insect pests by initiating breakdown of the secondary metabolites glucosinolates into toxic products. Several forms of myrosinases are present in plants but the properties and role of different isoenzymes are not well understood. The dicot plant model organism Arabidopsis thaliana seems to contain six myrosinase genes (TGG1–TGG6). In order to compare the different myrosinases, cDNAs corresponding to TGG1 from leaves and TGG4 and TGG5 from roots were cloned and overexpressed in Pichia pastoris. The His-tagged recombinant proteins were purified using affinity chromatography and the preparations were homogenous according to SDS–PAGE analysis. Myrosinase activity was confirmed for all forms and compared with respect to catalytic activity towards the allyl-glucosinolate sinigrin. There was a 22-fold difference in basal activity among the myrosinases. The enzymes were active in a broad pH range, are rather thermostable and active in a wide range of salt concentrations but sensitive to high salt concentrations. The myrosinases showed different activation–inhibition responses towards ascorbic acid with maximal activity around 0.7–1 mM. No activity was registered towards desulphosinigrin and this compound did not inhibit myrosinase activity towards sinigrin. All myrosinases also displayed O-β-glucosidase activity, although with lower efficiency compared to the myrosinase activity. The differences in catalytic properties among myrosinase isozymes for function in planta are discussed.