里氏木霉分泌型表达载体的构建及绿色荧光蛋白的表达

【目的】构建里氏木霉分泌型表达载体,通过表达绿色荧光蛋白论证载体的可行性并初步观察绿色荧光蛋白在里氏木霉中的分泌过程。【方法】应用PCR及分子克隆技术将里氏木霉(Trichoderma reesei)纤维二糖水解酶(CBH1)的启动子及CBH1自身信号肽、终止子和潮霉素筛选基因依次插入骨架质粒pUC19中,构建出T.reesei表达载体Ppth15。将增强型绿色荧光蛋白(eGFP)基因装载入Ppth15中,获得eGFP表达载体Ppth15-eGFP。再将Ppth15-eGFP转化进T.reesei原生质体,通过潮霉素抗性筛选、基因组PCR检测等方法鉴定,获得阳性重组转化子。【结果】用PDA培养基培养阳性转化子2-3 d后,可在菌丝顶端、隔膜及培养基中清晰地观察到大量绿色荧光。【结论】表达载体构建成功且能够用于eGFP的表达,实验为进一步研究T.reesei表达其他基因提供了有效工具,同时为T.reesei胞外蛋白分泌的研究提供了参考。     

Dolichol phosphate mannose synthase from the filamentous fungus Trichoderma reesei belongs to the human and Schizosaccharomyces pombe class of the enzyme

Dolichol phosphate mannose (DPM) synthase activity, which is required in N:-glycosylation, O-mannosylation, and glycosylphosphatidylinositol membrane anchoring of protein, has been postulated to regulate the Trichoderma reesei secretory pathway. We have cloned a T.reesei cDNA that encodes a 243 amino acid protein whose amino acid sequence shows 67% and 65% identity, respectively, to the Schizosaccharomyces pombe and human DPM synthases, and which lacks the COOH-terminal hydrophobic domain characteristic of the Saccharomyces cerevisiae class of synthase. The Trichoderma dpm1 (Trdpm1) gene complements a lethal null mutation in the S.pombe dpm1(+) gene, but neither restores viability of a S.cerevisiae dpm1-disruptant nor complements the temperature-sensitivity of the S. cerevisiae dpm1-6 mutant. The T.reesei DPM synthase is therefore a member of the "human" class of enzyme. Overexpression of Trdpm1 in a dpm1(+)::his7/dpm1(+) S.pombe diploid resulted in a 4-fold increase in specific DPM synthase activity. However, neither the wild type T. reesei DPM synthase, nor a chimera consisting of this protein and the hydrophobic COOH terminus of the S.cerevisiae DPM synthase, complemented an S.cerevisiae dpm1 null mutant or gave active enzyme when expressed in E.coli. The level of the Trdpm1 mRNA in T.reesei QM9414 strain was dependent on the composition of the culture medium. Expression levels of Trdpm1 were directly correlated with the protein secretory capacity of the fungus.     

The copper transport protein Atox1 promotes neuronal survival

Atox1, a copper transport protein, was recently identified as a copper-dependent suppressor of oxidative damage in yeast lacking superoxide dismutase. We have previously reported that Atox1 in the rat brain is primarily expressed in neurons, with the highest levels in distinct neuronal subtypes that are characterized by their high levels of metal, like copper, iron, and zinc. In this report, we have transfected the Atox1 gene into several neuronal cell lines to increase the endogenous level of Atox1 expression and have demonstrated that, under conditions of serum starvation and oxidative injury, the transfected neurons are significantly protected against this stress. This level of protection is comparable with the level of protection seen with copper/zinc superoxide dismutase and the anti-apoptotic gene bcl-2 that had been similarly transfected. Furthermore, neuronal cell lines transfected with a mutant Atox1 gene, where the copper binding domain has been modified to prevent metal binding, do not afford protection against serum starvation resulting in apoptosis. Therefore, Atox1 is a component of the cellular pathways used for protection against oxidative stress.