烟曲霉钙调蛋白的红色荧光蛋白标记及其在菌株极性生长的动态分布

doi:10.3760/cma.j.issn.0412-4030.2018.01.011

中华皮肤科杂志 ›› 2018, Vol. 51 ›› Issue (1): 43-47.doi: 10.3760/cma.j.issn.0412-4030.2018.01.011

烟曲霉钙调蛋白的红色荧光蛋白标记及其在菌株极性生长的动态分布

曾荣¹,童建波¹,刘宇甄¹,陈青²,段志敏¹,刘彩霞¹,吕桂霞³,林彤³,李岷³

1. 中国医学科学院皮肤病研究所
2. 江苏省血液中心
3. 南京中国医学科学院北京协和医学院皮肤病研究所

收稿日期:2017-02-24 修回日期:2017-08-03 出版日期:2018-01-15 发布日期:2018-01-11
通讯作者: 李岷 E-mail:drlimin@sina.cn
基金资助:
国家自然科学基金;国家自然科学基金;江苏省自然科学基金;北京协和医学院青年基金项目;国家重点基础研究发展计划（973）项目;中国医学科学院医学与健康科技创新工程项目;中国医学科学院医学与健康科技创新工程项目

Dynamic distribution of calmodulin labeled with red fluorescent protein in the polar growth of Aspergillus fumigatus

Received:2017-02-24 Revised:2017-08-03 Online:2018-01-15 Published:2018-01-11
Supported by:
National Nature Science Foundation of China;National Nature Science Foundation of China;Nature Science Foundation of Jiangsu Province of China;PUMC Youth Fund;National Basic Research Program（973 Program）of China;CAMS Innovation Fund for Medical Sciences;CAMS Innovation Fund for Medical Sciences

摘要/Abstract

摘要：

目的构建自身启动子调控、含有红色荧光蛋白（RFP）标记的钙调蛋白烟曲霉菌株，观察菌株生长过程中钙调蛋白的动态分布。方法设计烟曲霉钙调蛋白基因的两端侧翼序列，对两序列及含有RFP-烟曲霉pyrG 营养标记（mRFP?AfpyrG）的质粒分别进行PCR扩增，再通过融合PCR对上述3个片段进行整合，形成转化用的线性片段。随后采用原生质体转化法将上述片段转入烟曲霉受体菌株中，构建钙调蛋白-RFP烟曲霉菌株。在营养筛选培养基平板上挑取单克隆菌落培养，选取荧光表型最稳定的单菌菌落对其转化子进行PCR验证。将重组菌株和野生菌株分别接种于固体营养培养基中，培养不同时间后荧光显微镜下观察菌株形态学差异。将上述两株菌分别接种于液体培养基中，甲基四氮盐（XTT）方法观察其生长活力差异，并对红色荧光标记菌株进行动态活体观察，分析钙调蛋白在烟曲霉生长发育过程中的时空分布。结果重组菌株的荧光表型及转化子的PCR鉴定结果表明，钙调蛋白-RFP烟曲霉菌株构建成功。重组菌株与野生菌株在24 h时生长活力（A490值）分别为0.689 ± 0.081和0.678 ± 0.054（t = 1.32，P＞0.05），差异无统计学意义，且形态学方面也无显著差异。钙调蛋白在烟曲霉生长过程中始终处于极性生长过程中的菌丝顶端、分枝出芽点及新形成的分枝顶端。结论钙调蛋白可能参与调控烟曲霉孢子萌发及菌丝极性生长等重要生物学过程。

Abstract:

Zeng Rong, Tong Jianbo, Liu Yuzhen, Chen Qing, Duan Zhimin, Liu Caixia, Lyu Guixia, Lin Tong, Li Min Laser Department, Hospital of Dermatology, Chinese Academy of Medical Sciences and Peking Union Medical College, Jiangsu Key Laboratory of Molecular Biology for Skin Diseases and STIs, Nanjing 210042, China （Zeng R, Liu YZ, Lin T）; Department of Mycology, Hospital of Dermatology, Chinese Academy of Medical Sciences and Peking Union Medical College, Jiangsu Key Laboratory of Molecular Biology for Skin Diseases and STIs, Nanjing 210042, China （Tong JB, Duan ZM, Liu CX, Lyu GX, Li M）; Jiangsu Province Blood Center （Chen Q） Corresponding authors: Lin Tong, Email: ddlin@hotmail.com; Li Min, Email: drlimin@sina.cn 【Abstract】 Objective To construct a native promoter-regulated Aspergillus fumigatus strain containing red fluorescent protein-labeled calmodulin（CaM-RFP）, and to observe the dynamic distribution of calmodulin during the growth of Aspergillus fumigatus. Methods Bilateral flanking sequences of Aspergillus fumigatus calmodulin gene were designed, and plasmids containing the two flanking sequences and mRFP-Aspergillus fumigatus pyrG gene （mRFP-AfpyrG） were amplified separately. The final linear PCR product for transformation was generated from the above three PCR products by fusion PCR. Then, the above linear fragment was transferred into the Aspergillus fumigatus strain by protoplast transformation, so as to construct the CaM-RFP Aspergillus fumigatus strain. The monoclonal colony was picked from the screening medium and subjected to culture. Then, the stablest fluorescent monoxenic strain of Aspergillus fumigatus was selected, and the transformant was verified by PCR. The recombinant strain and wild-type stain were cultured on solid nutrient media separately, and the morphology of these strains was observed by fluorescence microscopy at different time points. Additionally, the above 2 strains were cultured in liquid media separately, and XTT assay was performed to evaluate the growth activity of strains. Microscopy was also conducted to dynamically observe the CaM-RFP Aspergillus fumigatus strain, and analyze the spatial and temporal distribution of calmodulin during the growth and development of Aspergillus fumigatus. Results The fluorescent phenotype and PCR identification results both indicated the successful construction of the CaM-RFP Aspergillus fumigatus strain. The growth activity at 24 hours did not differ between the recombinant strain and wild-type stain （A490: 0.689 ± 0.081 vs. 0.678 ± 0.054, t = 1.32, P > 0.05）, so did the morphology. During the polarized growth of Aspergillus fumigatus, calmodulin was always at the top of the hyphae, germination site of the hyphal branch and the top of new branches. Conclusion Calmodulin may be involved in the regulation of spore germination and polar hyphal growth of Aspergillus fumigatus.

曾荣童建波刘宇甄陈青段志敏刘彩霞吕桂霞林彤李岷. 烟曲霉钙调蛋白的红色荧光蛋白标记及其在菌株极性生长的动态分布[J]. 中华皮肤科杂志, 2018, 51(1): 43-47.

参考文献 12

［1］	Ellis M, Richardson M, de Pauw B. Epidemiology［J］. Hosp Med, 2000, 61（9）: 605⁃609. DOI: 10.12968/hosp.2000.61.9.1415.<br />
［2］	Berridge MJ, Lipp P, Bootman MD. The versatility and universality of calcium signalling［J］. Nat Rev Mol Cell Biol, 2000, 1（1）: 11⁃21. DOI: 10.1038/35036035.<br />
［3］	Carafoli E. Calcium signaling: a tale for all seasons［J］. Proc Natl Acad Sci U S A, 2002, 99（3）: 1115⁃1122. DOI: 10.1073/pnas.032427999.<br />
［4］	Chin D, Means AR. Calmodulin: a prototypical calcium sensor［J］. Trends Cell Biol, 2000, 10（8）: 322⁃328. DOI: 10.1016/S0962⁃8924（00）01800⁃6.<br />
［5］	Itadani A, Nakamura T, Hirata A, et al. Schizosaccharomyces pombe calmodulin, Cam1, plays a crucial role in sporulation by recruiting and stabilizing the spindle pole body components responsible for assembly of the forespore membrane［J］. Eukaryot Cell, 2010, 9（12）: 1925⁃1935. DOI: 10.1128/EC.00022⁃10.<br />
［6］	Chen S, Song Y, Cao J, et al. Localization and function of calmodulin in live⁃cells of Aspergillus nidulans［J］. Fungal Genet Biol, 2010, 47（3）: 268⁃278. DOI: 10.1016/j.fgb.2009.12.008.<br />
［7］	Zeng R, Li M, Chen Q, et al. In vitro analyses of mild heat stress in combination with antifungal agents against Aspergillus fumigatus biofilm［J］. Antimicrob Agents Chemother, 2014, 58（3）: 1443⁃1450. DOI: 10.1128/AAC.01007⁃13.<br />
［8］	Kuhn DM, Balkis M, Chandra J, et al. Uses and limitations of the XTT assay in studies of Candida growth and metabolism［J］. J Clin Microbiol, 2003, 41（1）: 506⁃508. DOI: 10.1128/JCM.41.1. 506⁃508.2003.<br />
［9］	Sabuquillo P, Gea A, Matas IM, et al. The use of stable and unstable green fluorescent proteins for studies in two bacterial models: Agrobacterium tumefaciens and Xanthomonas campestris pv. campestris［J］. Arch Microbiol, 2017, 199（4）: 581⁃590. DOI: 10.1007/s00203⁃016⁃1327⁃0.<br />
［10］	Brand A, Vacharaksa A, Bendel C, et al. An internal polarity landmark is important for externally induced hyphal behaviors in Candida albicans［J］. Eukaryot Cell, 2008, 7（4）: 712⁃720. DOI: 10.1128/EC.00453⁃07.<br />
［11］	Wilson D, Mayer FL, Miramón P, et al. Distinct roles of Candida albicans⁃specific genes in host⁃pathogen interactions［J］. Eukaryot Cell, 2014, 13（8）: 977⁃989. DOI: 10.1128/EC.00051⁃14.<br />
［12］	Brand A. Hyphal growth in human fungal pathogens and its role in virulence［J］. Int J Microbiol, 2012, 2012: 517529. DOI: 10.1155/2012/517529.<br />

烟曲霉钙调蛋白的红色荧光蛋白标记及其在菌株极性生长的动态分布

Dynamic distribution of calmodulin labeled with red fluorescent protein in the polar growth of Aspergillus fumigatus

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