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表达人源HPD基因对酿酒酵母孢子壁二酪氨酸层正确组装的干扰 被引量:1
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作者 王晓文 殷政 +1 位作者 高晓冬 中西秀树 《食品与发酵工业》 CAS CSCD 北大核心 2019年第15期17-23,共7页
研究人类基因4-羟苯丙酮酸二加氧酶(4-hydroxyphenylpyruvate dioxygenase,HPD)的表达对酿酒酵母( Saccharomyces cerevisiae )产孢过程及酵母孢子壁组装的影响。将 HPD 导入酿酒酵母中,比较人源化 HPD 酵母与野生型酵母的表型差异,分析... 研究人类基因4-羟苯丙酮酸二加氧酶(4-hydroxyphenylpyruvate dioxygenase,HPD)的表达对酿酒酵母( Saccharomyces cerevisiae )产孢过程及酵母孢子壁组装的影响。将 HPD 导入酿酒酵母中,比较人源化 HPD 酵母与野生型酵母的表型差异,分析 HPD 对酵母产孢及孢子壁的影响。与野生型酵母相比,人源化 HPD 酵母对产孢率无影响,但孢子自身荧光强度下降,乙醚敏感性增加,荧光增白剂(calcofluor white,CFW)染色荧光强度增强,该结果表明孢子壁出现缺陷,其二酪氨酸层组装过程中部分缺失。进一步研究发现,人源化 HPD 酵母产孢时,Hpd蛋白的催化产物尿黑酸(homogentisate,HGA)在产孢过程中会被氧化从而引起培养基颜色变化,且二酪氨酸复合物会大量泄漏至培养基中,最终导致二酪氨酸层不能正确组装。该研究结果为酿酒酵母二酪氨酸层的形成机制提供了新的认知。 展开更多
关键词 酿酒酵母 4-羟苯丙酮酸二加氧酶(hpd) 产孢子 二酪氨酸层 氧化性 组装
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The structure of 4-hydroxylphenylpyruvate dioxygenase complexed with 4-hydroxylphenylpyruvic acid reveals an unexpected inhibition mechanism 被引量:1
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作者 Xiaoning Wang Hongyan Lin +5 位作者 Junjun Liu Xinyun Zhao Xi Chen Wenchao Yang Guangfu Yang Chang-guo Zhan 《Chinese Chemical Letters》 CSCD 2021年第6期1920-1924,共5页
4-Hydroxyphenylpyruvate dioxygenase(HPPD)is an important target for both drug and pesticide discovery.As a typical Fe(II)-dependent dioxygenase,HPPD catalyzes the complicated transformation of 4-hydroxyphenylpyruvic a... 4-Hydroxyphenylpyruvate dioxygenase(HPPD)is an important target for both drug and pesticide discovery.As a typical Fe(II)-dependent dioxygenase,HPPD catalyzes the complicated transformation of 4-hydroxyphenylpyruvic acid(HPPA)to homogentisic acid(HGA).The binding mode of HPPA in the catalytic pocket of HPPD is a focus of research interests.Recently,we reported the crystal structure of Arabidopsis thaliana HPPD(At HPPD)complexed with HPPA and a cobalt ion,which was supposed to mimic the pre-reactive structure of At HPPD-HPPA-Fe(II).Unexpectedly,the present study shows that the restored At HPPD-HPPA-Fe(II)complex is still nonreactive toward the bound dioxygen.QM/MM and QM calculations reveal that the HPPA resists the electrophilic attacking of the bound dioxygen by the trim of its phenyl ring,and the residue Phe381 plays a key role in orienting the phenyl ring.Kinetic study on the F381 A mutant reveals that the HPPD-HPPA complex observed in the crystal structure should be an intermediate of the substrate transportation instead of the pre-reactive complex.More importantly,the binding mode of the HPPA in this complex is shared with several well-known HPPD inhibitors,suggesting that these inhibitors resist the association of dioxygen(and exert their inhibitory roles)in the same way as the HPPA.The present study provides insights into the inhibition mechanism of HPPD inhibitors. 展开更多
关键词 4-hydroxyphenylpyruvate dioxygenase QM/MM calculation Potential surface scan Substrate self-inhibition
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Transcriptomic analysis of wheat reveals possible resistance mechanism mediated by Yr10 to stripe rust
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作者 Zhongyi Wu Gaohua Zhang +6 位作者 Ran Zhao Qi Gao Jinchen Zhao Xiaoxu Zhu Fangyan Wang Zhensheng Kang Xiaojing Wang 《Stress Biology》 2023年第1期477-494,共18页
Stripe rust,caused by Puccinia striiformis f.sp.tritici(Pst),is a catastrophic disease that threatens global wheat yield.Yr10 is a race-specific all-stage disease resistance gene in wheat.However,the resistance mechan... Stripe rust,caused by Puccinia striiformis f.sp.tritici(Pst),is a catastrophic disease that threatens global wheat yield.Yr10 is a race-specific all-stage disease resistance gene in wheat.However,the resistance mechanism of Yr10 is poorly characterized.Therefore,to elucidate the potential molecular mechanism mediated by Yr10,transcriptomic sequencing was performed at 0,18,and 48 h post-inoculation(hpi)of compatible wheat Avocet S(AvS)and incompatible near-isogenic line(NIL)AvS+Yr10 inoculated with Pst race CYR32.Respectively,227,208,and 4050 differentially expressed genes(DEGs)were identified at 0,18,and 48 hpi between incompatible and compatible interaction.The response of Yr10 to stripe rust involved various processes and activities,as indicated by the results of Gene Ontology(GO)enrichment analysis and Kyoto Encyclopedia of Genes and Genomes(KEGG)pathway analysis.Specifically,the response included photosynthesis,defense response to fungus,metabolic processes related to salicylic acid(SA)and jasmonic acid(JA),and activities related to reactive oxygen species(ROS).Ten candidate genes were selected for qRT-PCR verification and the results showed that the transcriptomic data was reliable.Through the functional analysis of candidate genes by the virus-induced gene silencing(VIGS)system,it was found that the gene TaHPPD(4-hydroxyphenylpyruvate dioxygenase)negatively regulated the resistance of wheat to stripe rust by affecting SA signaling,pathogenesis-related(PR)gene expression,and ROS clearance.Our study provides insight into Yr10-mediated resistance in wheat. 展开更多
关键词 TRANSCRIPTOME Yr10 Virus-induced gene silencing system (VIGS)system 4-hydroxyphenylpyruvate dioxygenase HPPD
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