尖孢镰刀菌致病机理和化感作用研究进展

尖孢镰刀菌引起的枯萎病在生产中的防控相当困难。通过总结国内外相关文献,综述近年来有关尖孢镰刀菌致病机理和化感作用的研究进展。尖孢镰刀菌通过分泌毒素和细胞壁降解酶共同致病,谱系特异性区域的存在是其致病性强和宿主范围广的主要原因;在尖孢镰刀菌各专化型中已分离出大量致病相关基因;其他植物和拮抗微生物(木霉菌、丛枝菌根真菌、非致病性尖孢镰刀菌以及植物生长促生菌)可以分泌化感物质,作用于宿主植物和尖孢镰刀菌,直接抑制尖孢镰刀菌的生长或激活宿主植物的防御反应。未来有关尖孢镰刀菌致病机理研究应该在基因组测序基础上构建精细的遗传图谱;对化感作用的研究应当深入探讨分子机理,利用高通量测序等技术在转录组或蛋白组水平上明确宿主植物抗枯萎病相关基因,同时利用分子标记辅助育种来筛选新的抗枯萎病品种。     

几种尖孢镰刀菌专化型中SIX1、SIX4、SIX6、SIX8同源基因分析

尖孢镰刀菌在与寄主的相互作用中分泌几个特定的富含半胱氨酸的小分子量蛋白进入木质部中启动致病力,被称为SIX(secreted in xylem)蛋白,为明确其在不同寄主中的作用,本研究比较分析了几种尖孢镰刀菌专化型中SIX1、SIX4、SIX6、SIX8同源基因序列。根据已完成的尖孢镰刀菌古巴专化型1号(Foc1)与4号生理小种(Foc4)全基因组测序序列信息及相关SIX基因序列设计引物,应用PCR方法扩增分析56株尖孢镰刀菌古巴专化型与18株其它专化型及非致病型尖孢镰刀菌菌与其它种或属共21株菌株中的SIX1、SIX4、SIX6、SIX8基因。结果表明:设计的SIX1、SIX4、SIX6、SIX8基因引物均不能从非致病性尖孢镰刀菌与其它镰刀属种或其它属的菌株DNA中扩增出目的条带;SIX1基因的2个引物均能从供试的Foc菌株DNA中扩增出目的条带,同时可从部分其它专化型菌株DNA中扩增出目的条带;SIX4基因引物仅能从供试的尖孢镰刀菌番茄专化型与部分甘蓝专化型菌株DNA中扩增出目的条带;SIX6引物仅能从供试Foc1、Foc2、Foc4菌株DNA中扩增出目的条带;SIX8基因引物能从所有供试的致病尖孢镰刀菌中DNA扩增出目的条带。研究发现的SIX6基因序列提供了快速鉴定尖孢镰刀菌古巴专化型的检测方法,同时为深入研究尖孢镰刀菌各个专化型中SIX基因的功能奠定基础。     

小单孢菌(Micromonospora rosaria)DSM803全基因组测序及分析

小单孢菌(Micromonospora rosaria)DSM 803是一种高GC含量的革兰氏阳性放线菌,分离自美国德克萨斯州土壤,能够合成玫瑰霉素抗生素。目前,还没有相关研究报道Micromonospora rosaria的全基因组序列,这限制了代谢产物合成途径和比较基因组学等研究。本研究首次通过高通量测序技术对小单孢菌DSM803进行全基因组测序,使用Velvet软件进行组装拼接得到310个Contigs,整个基因组大小约7.38 Mbp,GC含量为73.4%,序列已提交至美国国立生物技术信息中心(NCBI)的Gen Bank数据库(LRQV00000000)。比较基因组学及玫瑰霉素合成途径相关基因分析结果显示:小单孢菌DSM 803在碳水化合物转运和代谢及信号转导功能方面要明显强于其它功能;玫瑰霉素生物合成基因簇由20个基因组成并分散于4个Contigs中。本研究首次报道了一株大环内酯类抗生素玫瑰霉素生产菌小单孢菌DSM 803的全基因组序列,分析了基因组基本特征,预测了次级代谢产物合成基因簇,探讨了玫瑰霉素生物合成途径,为后续的进一步代谢调控与合成生物学提供了理论基础。     

禾谷镰刀菌降解毒素基因Tri101的克隆和序列分析

禾谷镰刀菌Tri101基因编码的单端孢酶烯3-O-乙酰转移酶可通过加乙酰基的形式使禾谷镰刀菌产生的单族毒素(如DON)转变为较低的毒性。本研究利用RT-PCR技术从禾谷镰刀菌0623中扩增并克隆了Tri101基因的cDNA片段,测序结果表明,Tri101基因核苷酸序列阅读框架全长1356bp(GenBank序列号:GQ907236),编码451个氨基酸的多肽,推测分子量为49.45kD,等电点为5.14。氨基酸序列同源性比对结果表明,它与Kimura报道的禾谷镰刀菌Tri101氨基酸序列同源性最高,为99.56%,与其它13种镰刀菌的Tri101氨基酸序列的同源性分别为97.91%-75.68%。系统进化树分析结果表明,Fusarium graminearium0623与Fusarium sporotrichioides属于同一进化枝且与Fusarium asiaticum有较近的亲缘关系,而与F.oxysporum、F.moniliforme、F.nygamai、F.nisikadoi和F.decemcellulare的亲缘关系较远。     

香蕉枯萎病菌Fow1基因的克隆及序列分析

为了解Fow1基因在尖镰刀菌古巴专化型侵染香蕉过程中的作用,及其与尖镰刀菌古巴专化型生理小种1号和生理小种4号之间的致病力差异的关系,采用PCR和RT-PCR方法扩增了2个生理小种的Fow1基因,并对扩增产物进行了克隆测序及相似序列搜索和比对,还对基因编码的蛋白进行了结构预测和功能分析。研究结果表明2个生理小种Fow1基因开放阅读框均为957bp,编码318个氨基酸,基因序列和氨基酸序列差异小,而且两个生理小种Fow1基因所编码的蛋白均具有酵母线粒体载体蛋白典型的结构特征,推测Fow1基因可能为香蕉枯萎病菌在香蕉组织中定殖所必需。从Fow1基因序列及其编码蛋白的氨基酸序列看,2个生理小种致病力的差异与Fow1基因并无明显对应关系,这为进一步研究Fow1基因功能奠定了基础。     

尖孢镰孢菌果胶裂解酶基因家族鉴定及侵染表达模式分析

【背景】番茄枯萎病是番茄生产中常见的土传真菌病害。【目的】为鉴定番茄枯萎病基因组果胶裂解酶基因家族,明确该基因家族在侵染过程表达模式。【方法】采用生物信息学方法鉴定了番茄枯萎病尖孢镰孢菌(Fusarium oxysporum f. sp. Lycopersici)基因组内PEL基因家族,并分析了基因结构、染色体定位及三级结构,同时利用荧光定量PCR分析了FoPEL1-16基因在接种番茄根系的表达情况。【结果】番茄尖孢镰孢菌基因组内PEL基因家族成员有16个。氨基酸序列长度在163-548个氨基酸,信号肽长度在16-21个氨基酸。染色体定位分析表明16个基因在染色体上分布不均,分别定位在7条染色体上。根据基因结构和保守基序分析结果 16个基因可分为4类。进化分析表明该基因家族成员可聚成4支。三级结构预测结果显示同一家族存在相似结构域。荧光定量PCR分析结果表明Fo PEL基因在侵染过程表达水平明显上升。【结论】番茄尖孢镰孢菌基因组内果胶裂解酶以基因家族形式存在,其基因结构存在差异暗示了其功能多样性;FoPEL基因在侵染过程表达明显增强,说明其参与病原菌的致病性。本研究为解析尖孢镰孢菌致病基因功能分析及寄主病原互作提供了重要理论基础。     

一株重寄生枝孢菌的基因组测序及重寄生机制分析

【背景】枝孢菌SYC63是一株具有重寄生作用和抗菌活性的潜在生防菌株,目前尚无研究报道该菌株的全基因组序列,因此限制了其开发与利用。对该菌株进行基因组测序与分析,将进一步了解其重寄生的分子机制,为其在生物防治上的应用奠定研究基础。【目的】解析枝孢菌SYC63基因组序列信息,初步探究该菌的重寄生作用机制。【方法】利用二代高通量测序平台对枝孢菌SYC63进行全基因组测序,运用相关软件对其测序数据进行基因组组装、基因功能注释、预测次级代谢产物合成基因簇并分析重寄生相关的碳水化合物酶类基因等。【结果】基因组组装后共得到17个contigs,总长度为31 912 211 bp,GC含量为52.80%,预测到12 327个编码基因。其中,4 029、949和6 595个基因分别能在KEGG、COG和GO数据库中被注释到,同时还预测到25个次级代谢产物合成基因簇。对重寄生机制相关的碳水化合物酶类进行分析并与重寄生菌株(拟盘多毛孢菌、木霉及盾壳霉)比较,发现该菌具有较多的糖苷水解酶和糖脂酶基因,而且细胞壁降解酶类基因经锈菌孢子壁处理后在转录组测序中显著上调表达,初步分析了该菌与重寄生木霉在分子水平上的...     

西瓜连作病害机理及生物防治研究进展

西瓜枯萎病是西瓜栽培中常见的土传病害,由尖孢镰刀菌西瓜专化型(Fusarium oxysporum f.sp.niveum)侵染所致,会导致西瓜品质和产量降低,造成西瓜连作障碍,已成为西瓜生产的主要限制因素。目前关于西瓜枯萎病的综合防治已有较多报道。然而,对于西瓜枯萎的致病机理缺乏深入系统的总结。本文从尖孢镰刀菌在西瓜体内的侵染和定殖,尖孢镰刀菌分泌毒素对西瓜生长的影响以及西瓜连作对土壤生态的影响等方面,综述了尖孢镰刀菌导致西瓜连作障碍的可能机理,同时总结了国内外关于枯萎病生物防治的研究进展,为深入了解西瓜枯萎病及其防治提供了科学依据。     

尖孢镰刀菌古巴专化型MAPK FoSlt2敲除突变体的转录组分析

尖孢镰刀菌古巴专化型Fusarium oxysporum f. sp. cubense（FOC）是威胁香蕉生产的重要土传病原真菌。丝裂原活化蛋白激酶（mitogen-activated protein kinase,MAPK）FoSlt2信号通路在调控尖孢镰刀菌古巴专化型的生长发育、细胞壁完整性和致病性方面发挥着重要作用。为了揭示FoSlt2信号通路的致病机理和寻找农药靶标,本研究利用高通量RNA-seq技术对该病菌野生型菌株和FoSlt2敲除突变体菌株的转录组进行了比较分析,结果表明差异表达基因共有2 164个,其中上调表达基因有1 184个,下调表达基因有980个。Gene Ontology（GO）功能分析结果表明,差异表达基因主要参与在结合、催化分子功能组和代谢过程、细胞过程生物学通路中。KEGG 功能富集分析结果表明,差异基因主要参与戊糖和葡糖醛酸盐转换、氨基糖和核苷酸糖、氨基葡聚糖降解、磷酸肌醇和碳类物质代谢通路,说明这些通路与尖孢镰刀菌古巴专化型的生长发育和致病性相关。该研究为尖孢镰刀菌古巴专化型致病机制的阐明奠定了理论基础。     

小单孢菌(Micromonospora rifamycinica)AM105全基因组测序及分析

小单孢菌(Micromonospora rifamycinica)AM105是一种高GC含量的革兰氏阳性放线菌,分离自中国南海红树林沉积物,能够合成利福霉素类抗生素。目前,还没有相关研究报道Micromonospora rifamycinica的全基因组序列,这限制了代谢产物合成途径和比较基因组学等研究。本研究首次通过高通量测序技术对小单孢菌AM105进行全基因组测序,使用Velvet软件进行组装拼接得到388个Contigs,整个基因组大小约6.85 Mb,GC含量为73.1%,序列已提交至美国国立生物技术信息中心(NCBI)的Gen Bank数据库(LRMV01000000)。本研究同时对基因组序列进行了基因预测与功能注释、COG和GO聚类分析及次级代谢产物合成基因簇预测等,相关研究结果将为小单孢菌Micromonospora rifamycinica的功能基因组学研究提供基础数据。     

纳他霉素高产菌株Streptomyces gilvosporeus F607基因组及其生物合成基因簇分析

【背景】纳他霉素(Natamycin)是一种天然、广谱、高效的多烯大环内酯类抗真菌剂,褐黄孢链霉菌(Streptomyces gilvosporeus)是一种重要的纳他霉素产生菌。目前S. gilvosporeus基因组序列分析还未有报道,限制了该菌中纳他霉素及其他次级代谢产物合成及调控的研究。【目的】解析纳他霉素高产菌株S. gilvosporeus F607的基因组序列信息,挖掘其次级代谢产物基因资源,为深入研究该菌株的纳他霉素高产机理及生物合成调控机制奠定基础。【方法】利用相关软件对F607菌株的基因组序列进行基因预测、功能注释、进化分析和共线性分析,并预测次级代谢产物合成基因簇;对纳他霉素生物合成基因簇进行注释分析,比较分析不同菌种中纳他霉素生物合成基因簇的差异;分析预测S.gilvosporeusF607中纳他霉素生物合成途径。【结果】F607菌株基因组总长度为8482298bp,(G+C)mol%为70.95%,分别在COG、GO、KEGG数据库提取到5 062、4 428、5063个基因的注释信息。同时,antiSMASH软件预测得到29个次级代谢产物合成基因簇,其中纳他霉素基因簇与S.natalensis、S. chattanoogensis等菌株的纳他霉素基因簇相似性分别为81%和77%。除2个参与调控的sngT和sgnH基因和9个未知功能的orf基因有差异外,S. gilvosporeus F607基因簇中其他纳他霉素生物合成基因及其排列顺序与已知的纳他霉素基因簇高度一致。【结论】分析了S. gilvosporeus全基因组信息,预测了S. gilvosporeus F607中纳他霉素生物合成的途径,为从基因组层面上解析S. gilvosporeus F607菌株高产纳他霉素的内在原因提供了基础数据,为揭示纳他霉素高产的机理及工业化生产和未来新药的发现奠定了良好的基础。     

一株高产苯乳酸的古墓土壤葡糖醋杆菌FBFS97的全基因组测序与分析

【背景】苯乳酸(phenyllactic acid,PLA)是一种应用潜力巨大的天然广谱抑菌物质。本课题组前期分离得到一株高产PLA的醋酸菌(acetic acid bacteria,AAB)——葡糖醋杆菌(Gluconacetobacter sp.)FBFS97,但尚未鉴定到种,而且其产PLA的分子机理尚不清楚。【目的】确定FBFS97的种属关系,解析FBFS97的遗传信息,特别是与PLA产生相关的基因。【方法】采用光学显微镜和扫描电镜对FBFS97的菌体形态进行表征,通过16S rRNA基因序列分析对FBFS97进行分类鉴定,并以高效液相色谱分析苯丙氨酸对其产PLA的影响。在此基础上,对FBFS97进行全基因组测序、拼接和基因预测,并进行GO/COG聚类、KEGG代谢通路和VFDB毒力等分析,以及PLA生物合成途径的预测。【结果】根据16S rRNA基因序列的比对结果,结合形态学分析,该菌被鉴定为古墓土壤葡糖醋杆菌(Gluconacetobacter tumulisoli)。将1 000 mg/L苯丙氨酸添加到FBFS97液体培养基中,发酵液中PLA最高浓度可达400 mg/L,为对照组的8倍。该菌的基因组大小为3 988 308 bp,(G+C)mol%含量为66.62%,编码基因3 500个;KEGG代谢通路分析表明,该菌基因组中存在经莽草酸途径合成PLA的所有基因;VFDB毒力预测结果显示,该菌基因组中不存在产生毒素的相关基因。【结论】首次报道了一株高产PLA的AAB——古墓土壤葡糖醋杆菌FBFS97的全基因组序列信息,并发现该菌株的基因组中含有合成PLA的所有相关基因,为后续进一步研究FBFS97产生PLA的生物合成途径提供了理论依据。     

Genome-Wide Analysis of Mitogen-Activated Protein Kinase Gene Family in Maize

Mitogen-activated protein kinase (MAPK) cascades are universal signal transduction modules in plants. As the last component of the MAPK cascade (MAPKKK–MAPKK–MAPK), MAPK plays important roles in linking upstream kinases and downstream substrates. The MAPK proteins belong to a complex gene family in plants, with 20 MAPK genes in the Arabidopsis genome, 17 in the rice genome, and 21 in the poplar genome. Although the maize genome sequencing has been completed, no comprehensive study has been reported thus far for the MAPK gene family in maize. In this study, we identified 19 MAPK genes in maize. These ZmMPK genes belong to four groups (A–D) found in other plants. The phylogeny, chromosomal location, gene structure, and the functional relevancy of ZmMPK genes were analyzed. Moreover, we discuss the evolutionary divergence of MAPK genes in maize. Furthermore, we analyzed the expression profiles of ZmMPKs using the public microarray data and performed expression analyses in maize seedlings and adult plants. The data obtained from our study contribute to a better understanding of the complexity of MAPKs in plants and provide a useful reference for further functional analysis of MAPK genes in maize.     

Tomatinase from Fusarium oxysporum f. sp. lycopersici is required for full virulence on tomato plants

Saponin detoxification enzymes from pathogenic fungi are involved in the infection process of their host plants. Fusarium oxysporum f. sp lycopersici, a tomato pathogen, produces the tomatinase enzyme Tom1, which degrades alpha-tomatine to less toxic derivates. To study the role of the tom1 gene in the virulence of F. oxysporum, we performed targeted disruption and overexpression of the gene. The infection process of tomato plants inoculated with transformants constitutively producing Tom1 resulted in an increase of symptom development. By contrast, tomato plants infected with the knockout mutants showed a delay in the disease process, indicating that Tom1, although not essential for pathogenicity, is required for the full virulence of F. oxysporum. Total tomatinase activity in the disrupted strains was reduced only 25%, leading to beta(2)-tomatine as the main hydrolysis product of the saponin in vitro. In silico analysis of the F. oxysporum genome revealed the existence of four additional putative tomatinase genes with identities to tomatinases from family 3 of glycosyl hydrolases. These might be responsible for the remaining tomatinase activity in the Deltatom1 mutants. Our results indicate that detoxification of alpha-tomatine in F. oxysporum is carried out by several tomatinase activities, suggesting the importance of these enzymes during the infection process.     

A genomewide survey of developmentally relevant genes in Ciona intestinalis. V. Genes for receptor tyrosine kinase pathway and Notch signaling pathway

In the present survey, we identified most of the genes involved in the receptor tyrosine kinase (RTK), mitogen activated protein kinase (MAPK) and Notch signaling pathways in the draft genome sequence of Ciona intestinalis, a basal chordate. Compared to vertebrates, most of the genes found in the Ciona genome had fewer paralogues, although several genes including ephrin, Eph and fringe appeared to have multiplied or duplicated independently in the ascidian genome. In contrast, some genes including kit/flt, PDGF and Trk receptor tyrosine kinases were not found in the present survey, suggesting that these genes are innovations in the vertebrate lineage or lost in the ascidian lineage. The gene set identified in the present analysis provides an insight into genes for the RTK, MAPK and Notch signaling pathways in the ancient chordate genome and thereby how chordates evolved these signaling pathway.     

Bioinformatics analysis reveals disturbance mechanism of MAPK signaling pathway and cell cycle in Glioblastoma multiforme

Background & objectives

To analyze the reversal gene pairs and identify featured reversal genes related to mitogen-activated protein kinases (MAPK) signaling pathway and cell cycle in Glioblastoma multiforme (GBM) to reveal its pathogenetic mechanism.

Methods

We downloaded the gene expression profile GSE4290 from the Gene Expression Omnibus database, including 81 gene chips of GBM and 23 gene chips of controls. The t test was used to analyze the DEGs (differentially expressed genes) between 23 normal and 81 GBM samples. Then some perturbing metabolic pathways, including MAPK (mitogen-activated protein kinases) and cell cycle signaling pathway, were extracted from KEGG (Kyoto Encyclopedia of Genes and Genomes) pathway database. Cancer genes were obtained from the database of Cancer Gene Census. The reversal gene pairs between DEGs and cancer genes were further analyzed in MAPK and cell cycle signaling pathway.

Results

A total 8523 DEGs were obtained including 4090 up-regulated and 4433 down-regulated genes. Among them, ras-related protein rab-13(RAB13), neuroblastoma breakpoint family member 10 (NBPF10) and disks large homologue 4 (DLG4) were found to be involved in GBM for the first time. We obtained MAPK and cell cycle signaling pathways from KEGG database. By analyzing perturbing mechanism in these two pathways, we identified several reversal gene pairs, including NRAS (neuroblastoma RAS) and CDK2 (cyclin-dependent kinase 2), CCND1 (cyclin D1) and FGFR (fibroblast growth factor receptor). Further analysis showed that NRAS and CDK2 were positively related with GBM. However, FGFR2 and CCND1 were negatively related with GBM.

Interpretation & conclusions

These findings suggest that newly identified DEGs and featured reversal gene pairs participated in MAPK and cell cycle signaling pathway may provide a new therapeutic line of approach to GBM.     

Genetic basis of carotenoid overproduction in Fusarium oxysporum

The phytopathogenic fungus Fusarium oxysporum is a model organism in the study of plant-fungus interactions. As other Fusarium species, illuminated cultures of F. oxysporum exhibit an orange pigmentation because of the synthesis of carotenoids, and its genome contains orthologous light-regulated car genes for this biosynthetic pathway. By chemical mutagenesis, we obtained carotenoid overproducing mutants of F. oxysporum, called carS, with upregulated mRNA levels of the car genes. To identify the regulatory gene responsible for this phenotype, a collection of T-DNA insertional mutants obtained by Agrobacterium mediated transformation was screened for carotenoid overproduction. Three candidate transformants exhibited a carS-like phenotype, and two of them contained T-DNA insertions in the same genomic region. The insertions did not affect the integrity of any annotated ORFs, but were linked to a gene coding for a putative RING-finger (RF) protein. Based on its similarity to the RF protein CrgA from the zygomycete Mucor circinelloides, whose mutation results in a similar carotenoid deregulation, this gene (FOXG_09307) was investigated in detail. Its expression was not affected in the transformants, but mutant alleles were found in several carS mutants. A strain carrying a partial FOXG_09307 deletion, fortuitously generated in a targeted transformation experiment, exhibited the carS phenotype. This mutant and a T-DNA insertional mutant holding a 5-bp insertion in FOXG_09307 were complemented with the wild type FOXG_09307 allele. We conclude that this gene is carS, encoding a RF protein involved in down-regulation of F. oxysporum carotenogenesis.     

Trichothecene nonproducer Gibberella species have both functional and nonfunctional 3-O-acetyltransferase genes

The trichothecene 3-O-acetyltransferase gene (FgTri101) required for trichothecene production by Fusarium graminearum is located between the phosphate permease gene (pho5) and the UTP-ammonia ligase gene (ura7). We have cloned and sequenced the pho5-to-ura7 regions from three trichothecene nonproducing Fusarium (i.e., F. oxysporum, F. moniliforme, and Fusarium species IFO 7772) that belong to the teleomorph genus Gibberella. BLASTX analysis of these sequences revealed portions of predicted polypeptides with high similarities to the TRI101 polypeptide. While FspTri101 (Fusarium species Tri101) coded for a functional 3-O-acetyltransferase, FoTri101 (F. oxysporum Tri101) and FmTri101 (F. moniliforme Tri101) were pseudogenes. Nevertheless, F. oxysporum and F. moniliforme were able to acetylate C-3 of trichothecenes, indicating that these nonproducers possess another as yet unidentified 3-O-acetyltransferase gene. By means of cDNA expression cloning using fission yeast, we isolated the responsible FoTri201 gene from F. oxysporum; on the basis of this sequence, FmTri201 has been cloned from F. moniliforme by PCR techniques. Both Tri201 showed only a limited level of nucleotide sequence similarity to FgTri101 and FspTri101. The existence of Tri101 in a trichothecene nonproducer suggests that this gene existed in the fungal genome before the divergence of producers from nonproducers in the evolution of Fusarium species.     

基于网络药理学和分子对接探索桑白皮治疗糖尿病周围神经病变的潜在机制

本研究运用网络药理学和分子对接方法对中药桑白皮治疗糖尿病周围神经病变(DPN)的活性成分、潜在作用靶点和信号通路进行研究,探索桑白皮治疗DPN的可能作用机制。首先从中药系统药理学数据库(TCMSP)筛选出桑白皮的活性成分及靶点基因。通过GeneCards数据库及OMIM数据库筛选出DPN的疾病靶点基因,并用Cytoscape软件构建“药物-有效成分-靶基因-疾病”中药调控网络图。将有效成分靶标与疾病靶标上传到STRING数据库,构建蛋白互作网络图(PPI),并使用R语言对得到的PPI进行核心基因的筛选。运用R语言对关键靶点进行GO富集分析和KEGG通路富集分析。其次从活性成分及靶点基因中根据degree值筛选出前3个关键成分,并将该网络中的基因靶点以degree值高低进行排序,选择前3个核心靶点,然后从RCSB数据库下载相关蛋白的结构,使用Pymol软件去除溶剂分子与配体,使用AutoDock软件进行分子对接。最后通过酶联免疫吸附实验和荧光光谱实验验证网络药理学富集分析的结果。最终预测到31个桑白皮活性成分,312个活性成分相关靶点,120个桑白皮-糖尿病周围神经病变共同有效靶点。活性成分中度值最高的为槲皮素,其次为山柰酚。PPI网络核心基因为转录因子AP-1(JUN)、丝裂原活化蛋白激酶1(MAPK1)、转录因子p65(RELA)、丝氨酸-苏氨酸蛋白激酶1(AKT1)、白介素6(IL-6)等;GO富集分析显示会影响基因的转录、细胞因子表达和蛋白激酶活性等;KEGG通路富集分析显示AGE-RAGE信号通路、流体剪切力和动脉粥样硬化为显著性最高的通路,其次为卡波西肉瘤相关疱疹病毒感染、MAPK信号通路、人巨细胞病毒感染、TNF信号通路。分子对接结果显示关键成分中槲皮素与对应靶点具有较好的结合活性。酶联免疫吸附实验提示桑白皮能够降低IL-6和TNF-α的表达,荧光光谱实验证实桑白皮能够减少AGEs。可见中药桑白皮治疗糖尿病周围神经病变具有多成分、多靶点、多功能、多通路的作用特点,其潜在的作用机制可能与AGE-RAGE信号通路、肿瘤坏死因子信号通路等有关。     

木贼镰孢基因功能注释及比较基因组学分析

为挖掘木贼镰孢(Fusarium equiseti (Corda) Sacc.)的产毒基因及明确其进化关系,通过BLAST软件与GO、KEGG、COG、E职NOG、CAZy等14个数据库结合的方法对其全基因组进行功能注释并挖掘产毒基因,进行系统进化分析及运用色谱技术研究产毒基因的分泌规律;以麦根腐平脐蠕孢、燕麦镰孢、尖...