黑曲霉糖化酶基因表达调控的研究：I.高产及低产菌株糖化酶表达…

对黑曲霉高产菌株Ｔ２１和原始菌株３．７９５糖化酶的基因表达从菌体生长、酶形成动力学、ｇｌａＡ基因拷贝数、糖化酶ｍＲＮＡ含量及其稳定性等多个方面进行了分析和比较。Ｔ２１和３．７９５糖化酶的大量产生均自菌体生长的静止期开始。培养７２ｈ捂得的菌体浓度相同,但Ｔ２１产生的糖化酶量为３．７９５的１０￣１７倍,说明糖化酶产量的差异不是因生物量或酶起始合成期不同引起的,而是由于细胞内酶表达量不同引起的。Ｎｏｒｔ     

黑曲霉糖化酶基因表达调控的研究 Ⅰ.高产及低产菌株糖化酶表达的总体分析和比较

对黑曲霉(Aspergillus niger)高产菌株T21和原始菌株3.795糖化酶的基因表达从菌体生长、酶形成动力学、glaA基因拷贝数、糖化酶mRNA含量及其稳定性等多个方面进行了分析和比较。T21和3.795糖化酶的大量产生均自菌体生长的静止期开始。培养72h后,两者的菌体浓度相同,但T2l产生的糖化酶量为3.795的10～17倍,说明糖化酶产量的差异不是因生物量或酶起始合成期不同引起的,而是由于细胞内酶表达量不同引起的。Northern杂交显示T21总RNA中糖化酶mRNA含量为3.795的4.3～4.4倍.两菌株glaA基因拷贝数及糖化酶mRNA的稳定性分析结果排除了这两个因素的影响,因此T21糖化酶mRNA含量的增加主要是glaA基因转录水平提高的结果。T21与3.795之间糖化酶水平差异(10～17倍)与糖化酶mRNA水平差异(4.3～4.4倍)的不一致性,提示T21和3.795之间除转录水平外可能还存在着翻译水平上的差异(2～4倍)。此外,T21和3.795均存在着对糖化酶基因表达的碳源调控机制,根据两者在淀粉、麦芽糖和葡萄糖培养条件下所产生的mRNA比均为4:3:2,可以认为,这种调控作用发生在转录水平上,并且具有相同的调控方式。     

黑曲霉糖化酶基因表达调控的研究：Ⅱ.A.niger T21和3.795glaA基因 …

对糖化酶高产菌株Ａ．ｎｉｇｅｒＴ２１和原始菌株Ａ．ｎｉｇｅｒ３．７９５和ｇｌａＡ５′上游区的序列分析证明,两者在１．５ｋｂ的区域内有９个部位的碱基不同。为考察这些碱基差异是否是引起Ｔ２１ｇｌａＡ基因转录水平提高的原因,构建了以Ｔ２１和３．７９５ａｌａＡ基因转录调控区及Ａ．ｎｉｄｕｌａｎｓ ｔｒｐＣ基因终止子为表达元件的Ｅ．ｃｏｌｉ ｈｐｈ基因表达载体（ｐＸＨ１２和ｐＧＨ１）,用ｐＸＨ２和ｐＧＨ１分     

黑曲霉糖化酶高产和低产菌株糖化酶基因调控区的克隆及其分析比较

以PCR合成的糖化酶高产菌株黑曲霉(Asp. Niger)T21糖化酶基因5’近端非编码区588bp(EcoRI-BamHI)的序列为探针,从T21染色体DNA中克隆到近2.0kb的糖化酶基因5’端非编码区序列,并以此序列为探针从糖化酶低产菌株黑曲霉3.795(T21的诱变出发株)的染色体DNA中克隆到1.5kb的糖化酶基因5’端非编码区序列。该二序列的分析测定结果表明,其结构特征与文献报道的黑曲霉糖化酶基因5’端非编码区的基本一致,被称为“核心启动子”(Core promoter)的TATAAAT框及GCAAT框,分别在翻译起始点的-109bp及-178bp处。此外,在曲霉amdS,amyB基因中已发现有调控功能的CCAAT序列存在于-449bp和-799bp处。高产和低产菌株糖化酶基因5’端非编码区序列的分析比较结果表明,有9个部位的碱基发生了变化。此实验结果为进一步研究黑曲霉糖化酶基因在转录水平上的调控规律打下了基础。     

黑曲霉3.795glaA基因及其5'调控区的克隆和序列分析

黑曲霉Ｔ２１是由黑曲霉３．７９５经诱变育种获得的糖化酶高产菌株,为阐明其高产的分子机制,由黑曲霉３．７９５克隆了糖化酶结构基因及其５′旁侧序列,并与黑曲霉Ｔ２１的相应序列进行了比较．由黑曲霉３．７９５菌丝体分离染色体ＤＮＡ,Ｓｏｕｔｈｅｒｎ杂交分析表明,糖化酶结构基因位于～２．５ｋｂ的ＥｃｏＲⅠ－ＥｃｏＲⅤ染色体ＤＮＡ片段上,在此ＥｃｏＲⅠ位点上游约１．０ｋｂ处有一ＳａｌⅠ位点．为构建糖化酶结构基因及其５′旁侧序列的基因组文库,该染色体ＤＮＡ分别用ＥｃｏＲⅠ＋ＥｃｏＲⅤ和ＥｃｏＲ＋ＳａｌⅠ消化,琼脂糖凝胶电泳分离并回收长度在１．０ｋｂ左右和２．５ｋｂ左右的ＤＮＡ片段,分别与ｐＵＣ１９载体连接后转化入Ｅ．ｃｏｌｉＤＨ５．用原位杂交方法筛选到了携带糖化酶基因编码区及其１５０５ｂｐ５′旁侧序列的阳性克隆．对克隆片段的ＤＮＡ序列进行了测定并与黑曲霉Ｔ２１的相应序列进行了比较,结果表明,在糖化酶基因编码区及其１５０ｂｐ３′非编码区内,未发现碱基差异,但在－３４０～－１５０５的５′上游区内发生了９个位置的碱基变化,包括缺失、插入和替换．这些结果表明,黑曲霉Ｔ２１与３．７９５的糖化酶产量的差异与其结构基因无关,但可能与其     

丝状真菌表达分泌系统中受体菌的构建

黑曲霉糖化酶高产菌株T21经紫外诱变后, 通过酪蛋白平板和蛋白酶活性测定筛选出胞外酸性蛋白酶活力仅为原株076%的菌株A.nigerT21-201,其生长特性和产糖化酶活力与原株基本一致。利用原生质体PEG法将含有报告基因vhb的表达分泌质粒Pgt10-vhb通过与选择标记质粒的共转化导入此蛋白酶部分缺陷株及其原株T21,检测在蛋白酶缺陷株Aspergillus niger T21-201 和原株T21中VHb的分泌表达,结果表明在A.nigerT21-201中VHb表达水平显著高于原株,但Northern blot却显示在两菌株中^vnb基因的转录水平近似,由此证明酸性蛋白酶缺陷对保护外源蛋白产生了显著效果。      

Nucleotide sequence and expression of the glucoamylase-encoding gene (glaA) from Aspergillus oryzae.

The glucoamylase-encoding gene (glaA) from Aspergillus oryzae was cloned using its cDNA as a probe, which had been isolated previously. From comparison of nucleotide (nt) sequences of genomic clones with its cDNA, the glaA gene was found to contain four short putative introns, 45-56 nt in length. The A. oryzae glaA gene shared 62% homology at the nt level with the A. niger glaA gene with the four introns located at the same position. The 5'-flanking region contained a TATA box at nt-72 from the start codon, and two putative CAAT sequences at nt-87 and -331. Genomic Southern analysis and physical mapping showed that the glaA gene is located on the smallest chromosome (3.4 Mb) of six separated bands of chromosomes. Clones containing the glaA gene, when re-introduced intro A. oryzae, resulted in a three- to eightfold increase in glucoamylase activity.     

Glucoamylase overexpression and secretion in Aspergillus niger: analysis of glycosylation

We have studied the effects of overexpression and secretion of a homologous model glycoprotein, glucoamylase (GAM-1), on glycosylation in a single gene copy wild-type parent and multiple gene copy transformants of Aspergillus niger. In batch culture the B36 strain, which possess 80 additional copies of the GAM glaA gene, secreted about 5-8-fold more protein and GAM-1 than the parent strain (N402). A comparison of the glycosylation of GAM-1 secreted by the parent strain with that secreted by the multiple copy and hyper-secreting B36 strain showed that both the N-linked and O-linked glycan composition was very similar. Short oligomannose N-linked glycans were found (Man(7-8)GlcNAc(2)). O-Linked glycans were comprised of short (1-3 residues) oligosaccharide chains of mannose and galactose. Evidence is presented that this galactose is present in the novel galactofuranose conformation. This glycan composition of GAM-1 differed from that of a commercially available (A. niger) GAM source. Microsomes prepared from the mycelium showed a 2-3-fold co-ordinated increase in the activity of the dolichol phosphate:glycosyltransferases. Similar results were obtained from strains B1 (20 copies of glaA) and N402 when grown at a low dilution rate in a chemostat, although both the levels of GAM secretion and the activities of the dolichol phosphate:glycosyltransferases were lower than found in batch culture. These data suggest that A. niger is capable of secreting large amounts of a single glycoprotein combined with higher activity levels of the dolichol phosphate:glycosyltransferases without an increase in the heterogeneity of the glycan structures. Thus, from a biotechnological viewpoint, protein glycosylation may not be a bottleneck to enhanced glycoprotein production using A. niger.     

黑曲霉糖化酶基因上游调控区的克隆与分析

目的:通过基因工程方法改造糖化酶基因上游调控区,提高糖化酶产量提供研究。方法:以糖化酶生产菌黑曲霉为材料,通过PCR扩增获得糖化酶基因上游调控区片段PglaA。经测序比对发现该序列与GenBank中编号AM270061的序列相似性为100%。进一步的分析结果表明此序列含有2个保守的激活蛋白结合位点序列CCAAT和1个可能的葡萄糖阻遏位点CT-GGGG。结果:通过不同浓度葡萄糖对糖化酶合成的影响确定该菌株存在葡萄糖阻遏效应,当浓度到到3%以上时阻遏率高达70%以上,为葡萄糖阻遏位点预测结果提供了实验证据,并且经实验测得糖化酶活力随着接种量的增加而增加,当增加到5%时,相对酶活最高。     

强启动子glaA介导cbhB基因在黑曲霉中的表达

黑曲霉纤维素酶三类不同酶系中,纤维二糖水解酶基因表达处于很低水平,导致纤维素酶总体活力水平不高。为构建黑曲霉纤维素酶高产菌株,采用基因工程方法,全基因合成拼接黑曲霉高表达葡萄糖淀粉酶基因glaA的强启动子片段与纤维二糖水解酶基因cbhB编码区片段,然后将杂合基因克隆到二元载体pCAMBIA1301上,重组质粒通过农杆菌介导转化黑曲霉分生孢子,携带杂合基因的T-DNA片段插入到黑曲霉转化子的染色体上,共筛选到48个具有潮霉素抗性的转化子。纤维素酶活力水平测定结果显示,转化子A3-9的CMC酶活力最高,为野生型黑曲霉菌株的1.31倍;转化子B1-7与A3-6的滤纸酶活力最高,为野生型黑曲霉菌株2.51倍。另外,初步分析了杂合基因在黑曲霉中的表达所需的诱导条件。     

携多拷贝glaA的重组黑曲霉过量合成糖化酶的研究

以工业生产菌株黑曲霉CICIMF0410基因组DNA为模板,扩增出糖化酶glaA基因,测序并进行表达研究。GlaA基因的核苷酸序列长为2167bp,包含4个内含子。氨基酸序列比对表明此黑曲霉糖化酶与其他曲霉属来源的糖化酶有很高的同源性。将glaA基因克隆到pBC-Hygro载体中,构建重组质粒pBC-Hygro-glaA并转化A.nigerF0410。携多拷贝glaA的转化子用150μg/mL潮霉素抗性筛选并通过荧光实时定量PCR鉴定。结果表明,在染色体整合2~3倍糖化酶基因对糖化酶的过量合成是适宜的,有助于提高糖化酶活力。对转化子进行摇瓶发酵研究,发酵终止时转化子GB0506的糖化酶活力比出发菌株F0410提高了17.5%。因此,增加黑曲霉染色体糖化酶基因的拷贝数可以显著提高糖化酶活力。