近十年海洋来源木霉属真菌次生代谢产物研究进展

木霉（Trichoderma spp.）是一类自然界广泛存在于土壤中的真菌类群,属于半知菌门（Deuteromycotina）丝孢目（Moniliales）木霉属（Trichoderma sp.）。海洋中的木霉属真菌因其高盐、高压和缺氧的特殊环境,能够产生更多结构新颖、生物活性独特的次生代谢产物。木霉属真菌的次生代谢产物主要包括聚酮、肽类、萜类以及其他类型,这些化合物具有细胞毒、抗菌、酶抑制等多种生物活性。本文综述近十年来海洋来源木霉属真菌中分离的新次生代谢产物,并对这些新化合物的生物活性进行归纳总结。     

Construction of Streptomyces lydicus A01 transformant with the chit33 gene from Trichoderma harzianum CECT2413 and its biocontrol effect on Fusaria

Streptomyces lydicus A01 resists many plant pathogens (including Fusarium spp.) by producing the antifungal agent natamycin, which binds to the ergosterol of fungal cell membranes and inhibits the growth of pathogens. Trichoderma harzianum CECT2413 is a widely-distributed soil fungus that antagonizes several plant fungal pathogens (including Fusarium spp.) by producing chi-tinase and degrading chitin, a major component of the fungal cell wall. This study attempted to enhance the biocontrol effect of S. lydicus A01 on Fusarium spp. by transforming the chitinase gene of Trichoderma. Chitinase and natamycin could act synergisti-cally on both the cell walls and cell membranes of pathogens. The 33-kD chitinase-encoding gene (chit33) was cloned and conju-gal-transformed from T. harzianum CECT2413 to S. lydicus A01, and then confirmed via polymerase chain reaction (PCR) assays. Subsequent analyses using the 3,5-dinitrosalicylic acid (DNS) method and ultraviolet spectrophotometry showed that compared with its wild type strain (WT), the S. lydicus A01 conjugal transformant (CT) with chit33 gene exhibited substantially higher chi-tinase activity and natamycin production. The resistance of S. lydicus A01-chit33 CT and WT to four Fusaria in crops and vegetables was tested via the cup-plate method. Compared with the WT, the conjugal transformant of S. lydicus A01 with chit33 gene from T. harzianum CECT2413 showed greatly increased biocontrol effect on fusarium disease. This study would be beneficial to the development of high-quality antifungal bio-agents for agricultural applications via the synergy between the previously non-existent and pre-existing functions achieved through heterogeneous gene transformation.     

Cloning and expression of the vp39 gene of Bombyx mori nuclear polyhedrosis virus in E. coli

The nuclear capsid protein gene (vp39) ofBombyx mori nuclear polyhedrosis virus (BmNPV) was amplified successfully by PCR technique and inserted into pGEM 3zf(+). The 5′ and 3′ terminal area of the amplified vp39 gene were sequenced with silver-staining dideoxy method. Bmvp39 gene was sub-cloned into the expression vector pRSET-A, and transformed intoE. coli BL21. This gene was highly expressed by IPTG induction. SDS-PAGE analysis showed that the expressed protein is about 38 kd, and the expressed amount reached maxium in 4 h with IPTG induction. Supported by the National Natural science Foundation of China and the Doctoral Foundation of Edn carto Committee Liu Deli: born in 1954, Doctoral Candidate from Huazhong Normal University To whom correspondence should be addressed: (027-7882712-2938)     

Cloning and expression of the vp39 gene ofBombyx mori nuclear polyhedrosis virus inE. coli

The nuclear capsid protein gene (vp39) ofBombyx mori nuclear polyhedrosis virus (BmNPV) was amplified successfully by PCR technique and inserted into pGEM 3zf(+). The 5′ and 3′ terminal area of the amplified vp39 gene were sequenced with silver-staining dideoxy method. Bmvp39 gene was sub-cloned into the expression vector pRSET-A, and transformed intoE. coli BL21. This gene was highly expressed by IPTG induction. SDS-PAGE analysis showed that the expressed protein is about 38 kd, and the expressed amount reached maxium in 4 h with IPTG induction. Supported by the National Natural science Foundation of China and the Doctoral Foundation of Edn carto Committee Liu Deli: born in 1954, Doctoral Candidate from Huazhong Normal University To whom correspondence should be addressed: (027-7882712-2938)     

Expression of human β-subunit nerve growth factor (hNGFB) in yeast Pichia pastoris and E. coli

The gene hNGFB encoding the β subunit of human nerve growth factor (hNGF) was cloned intoP. pastoris secretive expression vector pHIL-S1 andE. coli expression vector pET-15b. The recombinant hNGFB vectors pSNGF and pET15b-NGF were transformed intoP. pastoris host cell GS115 (Mut⁺, His⁻) andE. coli strain BL21 (DE3) respectively. Expression and secretion of hNGFB inP. pastoris was attempted under the direction of the AOX1 promoter and PHO1 signal sequence. The positive colonies growing on medium without histidine were further selected by PCR. The yield of rehNGFB in GS115 was about 14.4% of total cellular secretive protein. The secreted protein was immunological active on Western blotting with rabbit anti-mNGFB antibodies. The fusion protein yield of rehNGFB inE. coli BL21 (DE3) was about 10.3% of total cellular protein after IPTG induction. Western blot detection showed its immunological activity.     

白蚁肠道木质素分解菌PY12的分离鉴定及lip基因的克隆

利用苯胺蓝平板法从白蚁肠道中分离到一株木质素分解高效菌株PY 12,经形态观察、生化鉴定和16 SrRNA鉴定为肠杆菌属的霍氏肠杆菌(Enterobacterhormaechei).根据已报道的lip(木质素过氧化物酶,Lignin Peroxidase)基因序列设计特异性引物,克隆该菌的lip基因,将其克隆入pMD19-T载体,获得的核苷酸序列为918 bp,并与GenBank中已知的lip序列进行同源性对比,同源性不高,但该核苷酸翻译后的氨基酸序列比对结果发现,其与假单胞杆菌Pseudomonas sp.编码蛋白质的氨基酸序列同源性为88.5%.     

5种药剂对银杏叶枯病菌的室内抑菌试验

在实验室中,用含药培养基法,抑菌圈法和孢子萌发法观测杀菌剂加瑞农,甲基托布津,多菌灵,可杀得,扑海因对银杏叶枯病的3种主要病原菌：细交链孢菌（Alternaria tenuis Ness),盘毛毛菌（Pestalotia ginkgo Hori),炭疽菌[Collelotrichum gloeosporioides(Penz)Sacc]的抑菌作用,结果表明,扑海因对细交链孢菌和盘多毛孢菌的菌落生长和孢子萌都有较强的抑制效果,对炭疽菌也有一定的抑制作用,甲基托布津和多菌灵对炭疽菌的抑制效果最好。     

Establishment ofChlamydomonas reinhardtii chloroplast expression

An expression vector pACⅢ containing the chimeric gene HAV- VP3P1 and HCV-C gene has been constructed and transferred to C. reinhardtii by the biolistic method. The trans-formants have been identified by PCR, Southern-blotting, Northern-blotting and Western-blotting assays after selecting on resistant medium and incubating in the dark. The results show that the chimeric gene has replaced the chIL gene of C. reinhardtii chloroplast genome and expressed correctly under the control of the C. reinhardtii chloroplast double promoters 5' chlL-5' atpA. The analysis of SDS-PAGE indicates that the expressed protein accounts for 5.31 % of total soluble protein.     

Expression and characterization of HGV E2 cDNA inPichia pastoris

A 559 base pair fragment of cDNA locating at the putative E2 region of GBV-C/HGV was inserted intoPichia pastoris expression vector pPIC9K in the reading frame of α-factor secreting signal peptide. The recombinant expression plasmid pPIC9K-E2 was introduced intoP. pastoris GS 115 with electroporation and recombined with the host genome by homological recombination. The His⁺Mut⁺ recombinant yeasts were selected and cultivated in the BMMY medium. After 3 days induction with 0.5% methanol, the target protein (E2) accumulated up to 30% of total proteins in the supernatant. The expressed E2 protein was proved possessing antigenicity and high specificity with Western blot and ELISA probed with sera from the immunized rabbits and the patients infected by GBV-C/HGV. Biography: Wang Zhuo-hua (1977-), female, Master, research direction: genetic engineering pharmaceuticals.     

海洋来源真菌的曲酸发酵条件优化

为提高真菌Aspergillus sp.GXIMD02003的曲酸产量,本研究对其利用大米固体培养基发酵的条件进行优化,旨在获得成本低廉的曲酸原料,促进曲酸的工业化生产。研究采用单因素控制变量法考察最佳盐度和最佳发酵时间,通过HPLC法测定曲酸的产量。结果表明真菌Aspergillus sp.GXIMD02003产曲酸的最佳发酵条件为在2%海盐的大米固体培养基中发酵30 d,在此条件下1 000 g大米培养基能够发酵产生24.2 g曲酸。因此,海洋来源真菌Aspergillus sp.GXIMD02003可以作为曲酸的生产菌株,海盐浓度影响该菌株的曲酸代谢。     

Molecular cloning, chromosomal mapping and expression analysis of disease resistance gene homologues in rice (Oryza sativa L.)

Resistance-like sequences have been amplified from first strand cDNA and genomic DNA of rice by PCR using oligonucleotide primers designed from sequence motifs conserved between resistance genes of tobacco andArabidopsis thaliana. 3 PCR clones, designatedOsr1, Osr2 andOsr3 which were 98% identical in nucleotide sequence level, have been found to be significantly homologous to known plant resistance genes and all contained the conserved motifs of NBS-LRR type resistance genes, such as P-loop, kinase2a, kinase3a and transmembrane domain.Southern hybridization revealed that rice resistance gene hornologueswere organized as a cluster in the genome. RFLP mapping using a DH population derived from anindica/japonka cross (Zhaiyeqing 8/Jingxi 17) and an RFLP linkage map assigned two copies ofOsrl and one copy ofOsr3 to the distal position of chromosome 12 where a blast resistance QTL has been mapped previously. Northern blot analysis showed thatOsrl gene was constitutively transcribed in rice leaves, shoots and roots. Further study concerning isolation of full-length cDNAs would be conducive to elucidating the functions of these genes.     

Molecular mapping of a novel yellow rust resistance gene of wheat using microsatellite markers

Identification and genetic analysis of yellow rust resistance have suggested that wheat line R55 carries single dominant gene conferring yellow rust resistance. The bulked segregant analysis (BSA) for an F₂ population using microsatellite marker technique has indicated that the yellow rust resistance gene is located on the short arm of chromosome 1B, tightly linked to the microsatellite markers WMS11-193 bp and WMS18-184 bp, the linkage distance between the markers and the gene is 1.9 cM. This gene has been formally namedYr26. It is inferred from the pedigree, resistance and gene locus analysis that theYr26 has been transferred fromTriticum turgidum L. and is different from the other known yellow rust resistance genes.     

Can other host species of cotton bollworm be non-Bt refuges to prolong the effectiveness of Bt-cotton?

The potential ecological risks ofBacillus thurigiensis (Bt) insecticides and Bt-crops have caused increasing concern since their commercial release in the field, among which pests’ resistance to Bt-crops is the major ecological risk. Refuge tactic, which can produce sensitive populations, has proved to be a key and sound resistance management strategy in USA and Australia; however, no tactics have been performed in China where Bt-cotton is mostly planted with other host crops of cotton bollworm. Genetic variation and gene flow among different host populations of the cotton bollwormHelicoverpa armigera were analyzed using PCR fingerprinting method. The results show that maize and castor-oil plant, as well as cotton can take effect as refuges to prevent resistance of cotton bollworm to Bt-cotton, while peanut and sesame are not as suitable for planting with Bt-cotton as refuges in the field as low gene flow was detected among populations on peanut, sesame and Bt cotton.     

生菜遗传转化受体系统的建立及鲑鱼降钙素基因的导入

以散叶生菜大速生(Lactuca sativa var.capatata L.)为试材，以MS为基本培养基。采用不同激素配比，确定生菜高效诱芽培养基为MS 0．1 mg／L6-BA 0．05mg／LNAA；抗生素敏感性试验表明，筛选培养基中适宜的卡那霉素选择压为75mg／L，抑菌剂羧苄青霉素的适宜质量浓度为300mg／L；通过根癌农杆菌介导的叶盘法将鲑鱼降钙素(sCT)基因转入大速生散叶生菜，PCR检测转化率达25．4％。     

Cloning and Characterization of the fecC Gene Necessary for Optimal Growth under Iron-Deficiency Conditions in the Cyanobacterium Anabaena sp. PCC 7120

The fecC gene encoding a putative iron (Ⅲ) dicitrate transporte rwas cloned from nitrogen-fixing cyanobacterium Anabaena sp. PCC 7120, and inactivated. The mutant grows normally in medium with NO3^- , NH1^- or without combined nitrogen. But in iron-deficient medium, the mutant grows slowly. Photosynthetic properties were compared between the mutant and the wildtype strain, the content of photosynthetic pigments in the mutant is lower than that of the wild-type. The results of RT-PCR experiments show that the fecC gene is expressed under iron-deficient conditions, but is not expressed under iron-replete conditions. These results revealed that fecC gene product is required for optimal growth under iron-deficient conditions in Anabaena sp. PCC 7120.     

Chromosomal location of yellow rust resistance gene(s) inTriticum aestivum-Lophopyrum elongatum substitution lines

A set ofT. aestivum-L. elongatum substitution lines were studied on yellow rust resistance at seedling stage, inheritance of the resistance and esterase-5 (Est-5) analysis. The results demonstrated thatL. elongatum carried a new yellow rust resistance gene(s), which was dominant and located on chromosome 3E ofL. elongatum. The biochemical locus encoding Est-5 was also located on chromosome 3E, and was tentatively named Est-E5, which was co-segregant with theYr gene(s) in wheat background. In addition, the transmission frequencies of chromosome 3E in 3A/3E and 3D/3E hybrids selfing were significantly higher than that of chromosome 3E in 3B/3E hybrid, which was probably due to the difference on genetic relationships among A, B, D and E genomes.     

分子标记辅助选育含有抗稻瘟病基因和软米基因两系不育系水稻新品系

以"浦软粳S"为转育亲本,利用分子标记辅助常规育种技术成功培育出含有Pi9,Pita,Pib和Pigm稻瘟病抗性基因及软米基因(Wx~(mq)),同时表现柱头外露率高的两系不育系水稻新品系"2179S"."2179S"不育系茎秆粗壮,矮杆大穗,株高为63.8 cm,柱头外露率平均为60%.研究结果为今后培育具有稻瘟病抗性的优质两系杂交水稻新组合提供不育系亲本.     

海绵Pseudoceratina sp.共栖细菌多样性及其抑制甘蔗鞭黑粉菌活性研究

【目的】探讨广西斜阳岛附近海域海绵共附生细菌的多样性,并筛选对甘蔗鞭黑粉菌有抑制作用的活性物质,为发现潜在的细菌新物种及开发农用生防菌肥奠定基础。【方法】采用稀释涂布法,通过6种复合营养分离培养基,从海绵Pseudoceratina sp.中分离可培养的共附生细菌。采取细菌形态学观察去除冗余,通过PCR扩增菌株的16SrRNA基因序列,并通过构建系统发育树分析物种多样性。采用牛津杯法进行抑制甘蔗鞭黑粉菌活性筛选实验。【结果】从海绵Pseudoceratina sp.中共分离到可培养细菌54株,经16SrRNA基因序列对比后,获得24株细菌,隶属于13科14属。其中,菌株BGMRC 2118与已发表有效菌株的16SrRNA基因序列的最高相似率为96.46%,可能为潜在新种。抑菌筛选实验结果显示,有8株细菌的发酵粗提物对甘蔗鞭黑粉菌具有很强的抑菌活性。【结论】广西斜阳岛附近海域中海绵共附生细菌具有较高的物种多样性,蕴藏着丰富的新物种资源,富含生物活性菌株。     

Tup1基因缺失对酿酒酵母耐高糖性状的影响

研究Tup1基因对酿酒酵母（Saccharomyces cerevisiae）细胞耐高糖性状的影响。利用Cre/loxP系统对单倍体细胞中的转录因子Tup1基因进行敲除,单倍体细胞复倍后研究基因缺失菌株的性状变化。结果表明,Tup1基因缺失虽然减弱了菌株的呼吸能力,但却增强了菌株在高浓度葡萄糖培养基中的生长和发酵能力。Tup1基因可能通过调节酿酒酵母细胞呼吸强度来调控细胞的高糖应激反应。     

1株碱杆菌属菌株的分离和鉴定

 从新疆采集的盐土样品中分离到1株革兰氏阳性、严格好氧、产孢、嗜盐细菌菌株YIM 012,对其进行了系统分类学研究.菌株YIM 012为杆菌,生长最适温度为28~45℃,最适pH 7.0~8.0,并能在70~250g/L的盐质量浓度中生长良好.其DNA的G+C的摩尔分数为39%,16S rRNA基因序列分析结果显示,该菌株与碱杆菌属Alkalibacillus salilacus(DSM 16460^T)亲缘关系最近,相似性达到99.6%,但与同属其它2个有效种间相似性低于96%.杂交结果显示其与A. salilacus亲缘关系低于20%,并且在生理生化方面也有差异.综合分析,确定该菌株为碱杆菌属的1个新种,将其命名为嗜盐碱杆菌(Alkalibacillus halophilus).