中国真菌学杂志
中國真菌學雜誌
중국진균학잡지
CHINESE JOURNAL OF MYCOLOGY
2014年
5期
257-263
,共7页
向耘%冉玉平%仝爱平%勾蓝图%王伟%代亚玲
嚮耘%冉玉平%仝愛平%勾藍圖%王偉%代亞玲
향운%염옥평%동애평%구람도%왕위%대아령
双向电泳%蛋白%糠秕马拉色菌
雙嚮電泳%蛋白%糠秕馬拉色菌
쌍향전영%단백%강비마랍색균
two-dimensional electrophoresis%protein%Malassezia furfur
目的:通过双向电泳及串联质谱技术鉴定糠秕马拉色菌酵母态及菌丝态差异蛋白,在蛋白水平探讨两态转化机制及致病机理。方法分别诱导糠秕马拉色菌标准株酵母态和菌丝态菌体,利用玻璃珠研磨和超声波破碎细胞壁,三氯乙酸/丙酮沉淀获取总蛋白。双向电泳分离蛋白,PDQuest软件比对找出差异蛋白点。电喷雾串联质谱对差异点进行肽段测序,用Mascot和NCBI的Blast软件经蛋白质数据库鉴定蛋白质。结果经双向电泳分离的糠秕马拉色菌酵母态、菌丝态蛋白各有800多个蛋白点、64个蛋白点表达量有3倍以上差异,其中11个为酵母态特有,9个菌丝态特有。在选取的40个差异点中,成功鉴定出22个点,共16个蛋白。经Mascot和Blast软件检索,有明确功能的蛋白中,肌动蛋白、丝切蛋白等9个蛋白在菌丝态上调,谷胱甘肽转移酶、细胞支架信号蛋白等5个蛋白下调。结论鉴定出16个蛋白分别与细胞代谢、运动、氧化应激等功能相关,为了解糠秕马拉色菌表型转换机制和致病机理提供重要信息。
目的:通過雙嚮電泳及串聯質譜技術鑒定糠秕馬拉色菌酵母態及菌絲態差異蛋白,在蛋白水平探討兩態轉化機製及緻病機理。方法分彆誘導糠秕馬拉色菌標準株酵母態和菌絲態菌體,利用玻璃珠研磨和超聲波破碎細胞壁,三氯乙痠/丙酮沉澱穫取總蛋白。雙嚮電泳分離蛋白,PDQuest軟件比對找齣差異蛋白點。電噴霧串聯質譜對差異點進行肽段測序,用Mascot和NCBI的Blast軟件經蛋白質數據庫鑒定蛋白質。結果經雙嚮電泳分離的糠秕馬拉色菌酵母態、菌絲態蛋白各有800多箇蛋白點、64箇蛋白點錶達量有3倍以上差異,其中11箇為酵母態特有,9箇菌絲態特有。在選取的40箇差異點中,成功鑒定齣22箇點,共16箇蛋白。經Mascot和Blast軟件檢索,有明確功能的蛋白中,肌動蛋白、絲切蛋白等9箇蛋白在菌絲態上調,穀胱甘肽轉移酶、細胞支架信號蛋白等5箇蛋白下調。結論鑒定齣16箇蛋白分彆與細胞代謝、運動、氧化應激等功能相關,為瞭解糠秕馬拉色菌錶型轉換機製和緻病機理提供重要信息。
목적:통과쌍향전영급천련질보기술감정강비마랍색균효모태급균사태차이단백,재단백수평탐토량태전화궤제급치병궤리。방법분별유도강비마랍색균표준주효모태화균사태균체,이용파리주연마화초성파파쇄세포벽,삼록을산/병동침정획취총단백。쌍향전영분리단백,PDQuest연건비대조출차이단백점。전분무천련질보대차이점진행태단측서,용Mascot화NCBI적Blast연건경단백질수거고감정단백질。결과경쌍향전영분리적강비마랍색균효모태、균사태단백각유800다개단백점、64개단백점표체량유3배이상차이,기중11개위효모태특유,9개균사태특유。재선취적40개차이점중,성공감정출22개점,공16개단백。경Mascot화Blast연건검색,유명학공능적단백중,기동단백、사절단백등9개단백재균사태상조,곡광감태전이매、세포지가신호단백등5개단백하조。결론감정출16개단백분별여세포대사、운동、양화응격등공능상관,위료해강비마랍색균표형전환궤제화치병궤리제공중요신식。
Objectives To identify differential proteins in the yeast and mycelial phases of Malassezia furfur by using the two-di-mensional electrophoresis(2-DE)protocol and tandem spectrum( MS/MS),and to understand the pathogenic mechanism of M. furfur and its morphological switching mechanism at protein level as well Methods The type strain of M. furfur was inoculated in the yeast and mycelial phase media respectively Vortexing with glass beads and ultrasonication were used to break up the cell wall into pieces,and trichloroacetate/acetone precipitation was applied to obtain the total proteins These proteins were separated and vis-ualized by 2-DE,analyzed by PDQuest soft to detect the differentially expressed protein spots Electrospray-tandem spectrum analy-sis combined with homology search by Mascot and NCBIˊs Blast was used to identify proteins Results The stable protein profiles from the mycelial and yeast phases were compared,more than 800 spots were detected respectively Of these,64 spots were regula-ted more than 3-fold,11 were identified only in the yeast phases and 9 were identified only in the mycelial phases Selected 40 dif-ferential spots,22 were identified,corresponding to 16 unique proteins In the identified proteins,9 proteins including actin,cofilin etc were up-regulated and 5 proteins including glutathione transferase,cytoskeletal signaling protein etc,were down-regulated in mycelial phase Conclusions Sixteen protein spots implicated in some cellular processes,such as metobalism,motility,oxidase stress etc were positively identified by experiencements and important information would be provided for understanding the mecha-nisms underlying phenotype transformation of M. furfur and its pathogenesis.