留言板

尊敬的读者、作者、审稿人, 关于本刊的投稿、审稿、编辑和出版的任何问题, 您可以本页添加留言。我们将尽快给您答复。谢谢您的支持!

姓名
邮箱
手机号码
标题
留言内容
验证码

不同富集培养方法对噬菌体PEf771的滴度影响

杨镕羽 宋飞 魏云林 杨向红 段开文 向盈盈

downloadPDF
文章导航 > 昆明医科大学学报  > 2022 >  43(2): 7-11
杨镕羽, 宋飞, 魏云林, 杨向红, 段开文, 向盈盈. 不同富集培养方法对噬菌体PEf771的滴度影响[J]. 昆明医科大学学报, 2022, 43(2): 7-11. doi: 10.12259/j.issn.2095-610X.S20220218
引用本文: 杨镕羽, 宋飞, 魏云林, 杨向红, 段开文, 向盈盈. 不同富集培养方法对噬菌体PEf771的滴度影响[J]. 昆明医科大学学报, 2022, 43(2): 7-11. doi: 10.12259/j.issn.2095-610X.S20220218
shu
Rongyu YANG, Fei SONG, Yunlin WEI, Xianghong YANG, Kaiwen Duan, Yingying XIANG. Effects of Different Accumulation Culture Methods on the Titer of Phage PEf771[J]. Journal of Kunming Medical University, 2022, 43(2): 7-11. doi: 10.12259/j.issn.2095-610X.S20220218
Citation: Rongyu YANG, Fei SONG, Yunlin WEI, Xianghong YANG, Kaiwen Duan, Yingying XIANG. Effects of Different Accumulation Culture Methods on the Titer of Phage PEf771[J]. Journal of Kunming Medical University, 2022, 43(2): 7-11. doi: 10.12259/j.issn.2095-610X.S20220218
shu

不同富集培养方法对噬菌体PEf771的滴度影响

doi: 10.12259/j.issn.2095-610X.S20220218
  • 1.

    昆明医科大学附属延安医院口腔科,云南 昆明 650031

  • 2.

    昆明医科大学第三附属医院微创介入科,云南 昆明 650106

  • 3.

    昆明理工大学生命科学与技术学院,云南 昆明 650500

基金项目: 国家自然科学基金资助项目(31860147);云南省高层次卫生计生技术人才培养资助项目(H-2018086)
详细信息
    作者简介:

    杨镕羽(1996~),女,白族,云南大理人,硕士研究生,主要从事口腔临床工作

    通讯作者:

    向盈盈,E- mail:25591394@qq.com

  • 中图分类号: R780.1;Q93-3

Effects of Different Accumulation Culture Methods on the Titer of Phage PEf771

  • 1.

    Dept. of Stomatology,Yan’an Hospital of Kunming City,Kunming Yunnan 650031

  • 2.

    Dept. of Minimally Invasive Intervention ,The Third Affiliated Hospital of Kunming Medical University,Kunming Yunnan 650106

  • 3.

    Faculty of Life Science and Technology, Kunming University of Science and Technology,Kunming Yunnan 650500,China

    摘要
  • 摘要:   目的  对比3种不同富集培养方法对噬菌体PEf771的滴度影响,探讨有效提高噬菌体PEf771滴度的方法。  方法  通过噬菌体PEf771/粪肠球菌E. faecalis YN771比例法、挖斑法和丝裂霉素C诱导法在E. faecalis YN771不同生长时期加入PEf771原液进行富集,来获得较高的PEf771的滴度。  结果  PEf771/ E. faecalis YN771 = 1∶3和挖斑法得出的PEf771的滴度较高,将这2种方法扩大培养后无明显差异(P > 0.05),且在24 h滴度达108 pfu/mL。丝裂霉素C诱导法未能明显提高PEf771的滴度。通过在E. faecalis YN771生长早期(OD600 = 0.3)和对数期(OD600 = 1)加入PEf771进行富集培养,前者培养6 h滴度高达1010 pfu/ml,24 h滴度仍保持1010 pfu/ml,达到了理想滴度。  结论  在E. faecalis YN771培养早期(OD600 = 0.3)加入PEf771以噬菌体/菌 = 1∶3的方法或挖斑法富集培养可有效提高PEf771的滴度,为研究E. faecalis YN771的噬菌体PEf771治疗E. faecalis YN771引起的感染提供了实验材料和依据。
    Abstract:   Objective  To compare the effects of three different enriching culture methods on the titer of phage PEf771, and discuss the methods to effectively improve the titer of phage PEf771.   Methods  Through phage PEf771/E. faecalis YN771 proportional method, spot digging method and mitomycin C induction method, phage PEf771 stock solution was added at E. faecalis YN771 different growth stages for enrichment to obtain a higher titer of phage PEf771.   Results  The titer of PEf771 obtained by PEf771/E. faecalis YN771 = 1∶3 and spot digging method was higher, there was no significant difference between the two methods after expanded culture (P > 0.05), and the titer reached 108 pfu/mL in 24 hours. Mitomycin C induction method could not significantly improve the titer of PEf771.PEf771 was added in the early growth stage (OD600 = 0.3) and logarithmic stage (OD600 = 1) of E. faecalis YN771 for enrichment culture. The titer of the former was 1010 pfu/mL after 6 hours of culture, and remained 1010 pfu/mL after 24 hours, reaching the ideal titer.   Conclusion  Adding PEf771 in the early stage of E. faecalis YN771 culture (OD600 = 0.3) and enriching culture with PEf771/E. faecalis YN771 = 1∶3 or spot digging method can effectively improve the titer of PEf771. It provides experimental materials and basis for the study of phage PEf771 of E. faecalis YN771 in the treatment of infection caused by E. faecalis YN771.
    • HTML全文

  • 表  1  不同方法富集噬菌体的滴度比较

    Table  1.   Comparison of titer of phage enriched by different methods

    实验分组噬菌体对数期粪肠球菌
    (OD = 1)(μL)    		新鲜BHI
    (mL)    		噬菌体∶菌24 h滴度
    (pfu/mL)    		48 h滴度
    (pfu/mL)    		72 h滴度
    (pfu/mL)
    200 μL 250 5 4∶5 0.9×107 3.6×107 1.5×106
    200 μL 500 5 1∶2.5 3.0×107 4.1×108 2.1×107
    400 μL 500 5 4∶5 1.3×107 8.0×107 7.4×106
    400 μL 250 5 8∶5 1.9×107 5.3×107 6.8×106
    100 μL 300 5 1∶3 4.6×107 1.2×109 6.1×108
    挖斑(2块) 1000 100 2.2×108 1.8×109 7.4×108
    下载: 导出CSV

    表  2  两种方法富集培养的滴度比较

    Table  2.   Comparison of enrichment culture by two methods

    实验分组噬菌体对数期粪肠球菌
    (OD = 1)(mL)    		新鲜BHI
    (mL)    		24 h滴度
    (pfu/mL)    		48 h滴度
    (pfu/mL)    		72 h滴度
    (pfu/mL)
    噬菌体:菌 = 1∶3 一组 10 mL 30 500 4.7×108 3.6×107 2.1×106
    噬菌体:菌 = 1∶3 二组 10 mL 30 500 1.1×108 0.5×107 0.4×106
    噬菌体:菌 = 1∶3 三组 10 mL 30 500 1.2×108 0.8×107 0.7×106
    噬菌体:菌 = 1∶3 四组 10 mL 30 500 2.2×108 1.0×107 0.9×106
    挖板法一组 挖斑(10块) 500 7.5×108 6.2×107 8.0×106
    挖板法二组 挖斑(10块) 500 5.3×108 4.2×107 2.8×106
    挖板法三组 挖斑(10块) 500 6.4×108 4.5×107 3.9×106
    挖板法四组 挖斑(10块) 500 7.6×108 6.0×107 4.2×106
    下载: 导出CSV

    表  3  丝裂霉素C诱导法对噬菌体滴度的影响

    Table  3.   Effects of mitonmycin C induction on phage titer

    实验分组24 h滴度(pfu/mL)48 h滴度(pfu/mL)
    加丝裂霉素C组3.2×1084.5×107
    对照组5.3×1082.9×107
    下载: 导出CSV

    表  4  E. faecalis YN771对数早期加入噬菌体富集

    Table  4.   Enrichment of PEf771 by E. faecalis YN771 at different culture phases

    实验分组6 h滴度(pfu/mL)24 h滴度(pfu/mL)
    对数生长早期组
    (OD600 = 0.3)    		 1.6×1010 1.3×1010
    对数生长期组
    (OD600 = 1)    		 5.1×106 2.4×108
    下载: 导出CSV
    • 参考文献(15)
  • [1] Beloin C,Renard S,Ghigo J M,et al. Novel approaches to combat bacterial biofilms[J]. Current Opinion in Pharmacology,2014,18(18):61-68.
    [2] Mohamed J A,Wenxiang H,Nallapareddy S R,et al. Influence of origin of isolates,especially endocarditis isolates,and various genes on biofilm formation by Enterococcus faecalis[J]. Infection Immunity,2004,72(6):3658. doi: 10.1128/IAI.72.6.3658-3663.2004
    [3] 王韧韬,刘又宁. 噬菌体治疗细菌感染的临床应用与进展[J]. 中华结核和呼吸杂志,2020,43(6):539-543. doi: 10.3760/cma.j.cn112147-20190718-00517
    [4] Ben-Zaken H,Kraitman R,Coppenhagen-Glazer S,et al. Isolation and Characterization of Streptococcus mutans Phage as a Possible Treatment Agent for Caries[J]. Viruses,2021,13(5):825. doi: 10.3390/v13050825
    [5] Khalifa L,Shlezinger M,Beyth S,et al. Phage therapy against Enterococcus faecalis in dental root canals[J]. Oral Microbiol,2016,8(1):32157. doi: 10.3402/jom.v8.32157
    [6] Sarker S A,Sultana S,Reuteler G,et al. Oral Phage Therapy of Acute Bacterial Diarrhea With Two Coliphage Preparations:A Randomized Trial in Children From Bangladesh[J]. E Bio Medicine,2016,4(C):124-137.
    [7] Melinda,Gindin,Hallie P,et al. Bacteriophage for Gastrointestinal Health (PHAGE) Study:Evaluating the Safety and Tolerability of Supplemental Bacteriophage Consumption[J]. Journal of the American College of Nutrition,2019,38(1):68-75.
    [8] Ooi M L,Drilling A J,Morales S,et al. Safety and Tolerability of Bacteriophage Therapy for Chronic Rhinosinusitis Due to Staphylococcus aureus[J]. JAMA Otolaryngology-Head & Neck Surgery,2019,145(8):723-729.
    [9] Fabijan A P,Lin R,Ho J,et al. Safety of bacteriophage therapy in severe Staphylococcus aureus infection[J]. Nature Microbiology,2020,5(3):465-472. doi: 10.1038/s41564-019-0634-z
    [10] Yingying,Xiang,Wenyu,Li,Fei,Song,Xianghong,Yang,Jing,Zhou,Hongbin,Yu,Xiuling,Ji,Yunlin,Wei. Biological characteristics and whole-genome analysis of the Enterococcus faecalis phage PEf771.[J]. Canadian Journal of Microbiology,2020,66(9):505-520. doi: 10.1139/cjm-2019-0336
    [11] Yoon B H,Chang H I. Genomic annotation for the temperate phage EFC-1,isolated from Enterococcus faecalis KBL101[J]. Archives of Virology,2015,160(2):601. doi: 10.1007/s00705-014-2263-4
    [12] John S G,Mendez C B,Deng L,et al. A simple and efficient method for concentration of ocean viruses by chemical flocculation[J]. Environ Microbiol Rep,2011,3(2):195-202. doi: 10.1111/j.1758-2229.2010.00208.x
    [13] Hurwitz B L,Deng L,Poulos B T,et al. Evaluation of methods to concentrate and purify ocean virus communities through comparative,replicated metagenomics[J]. Envior Microbiol,2012,15(5):1428-1440.
    [14] Uchiyama J,Rashel M,Maeda Y,et al. Isolation and characterization of a novel Enterococcus faecalis bacteriophage phiEF24C as a therapeutic candidate[J]. Fems Microbiology Letters,2008,278(2):200. doi: 10.1111/j.1574-6968.2007.00996.x
    [15] Parasion S,Kwiatek M,Mizak L,et al. Isolation and characterization of a novel bacteriopha-ge phi4D lytic against Enterococcus faecalis strains[J]. Curr Microbiol,2012,65(3):284-289. doi: 10.1007/s00284-012-0158-8
    • 相关文章(20)
  • [1] 李洁, 何媛, 吴春燕, 单斌, 郑瑞, 管志福, 任宝军, 师春霞, 周友全, 刘涵禹, 张米, 康燕明, 宋贵波.  2017年—2021年云南地区无菌体液细菌的分布特征及耐药性分析, 昆明医科大学学报. doi: 10.12259/j.issn.2095-610X.S20230309
    [2] 王群, 孙雨欣, 王海峰.  脂滴表面蛋白perilipin家族在癌症中的研究进展, 昆明医科大学学报. doi: 10.12259/j.issn.2095-610X.S20230812
    [3] 杜钰娟, 陈华英, 田晓芳, 李玉婷, 姚静雯, 赵明月, 张丽芬.  类风湿关节炎患者出院准备度现状及影响因素, 昆明医科大学学报. doi: 10.12259/j.issn.2095-610X.S20220603
    [4] 张国庆, 周佳, 颜芮, 张冰, 李琳蓉, 李丽, 潘颖.  滇西贫困山区公共卫生服务能力的满意度现状, 昆明医科大学学报. doi: 10.12259/j.issn.2095-610X.S20210811
    [5] 向盈盈, 宋飞, 杨向红, 周静, 于鸿滨, 魏云林, 季秀玲.  噬菌体疗法在口腔感染性疾病中的应用, 昆明医科大学学报.
    [6] 王维波, 金永梅, 杨俊婕, 钱丽芳, 房梅芹, 白劲松.  艾滋病科应用移动护士站满意度分析, 昆明医科大学学报.
    [7] 李秀娟, 李玲妍, 李夏, 孔虹倩, 冉凌云.  临时性造口患者与永久性造口患者适应度对比, 昆明医科大学学报.
    [8] 胡万芹, 赵洪波, 梁宏, 赵庆华, 杨丽华.  顺铂耐药卵巢癌的差异表达基因和信号通路富集分析, 昆明医科大学学报.
    [9] 李辉, 王智, 辛应朋, 杨晓佩, 张柠, 赵斐, 钟树荣.  不同载体上人体脱落细胞富集方法的比较, 昆明医科大学学报.
    [10] 胡凤婵.  共情护理对剖宫产产妇焦虑情绪及护理满意度的影响, 昆明医科大学学报.
    [11] 张敏.  成都市某主城区社区卫生服务满意度调查, 昆明医科大学学报.
    [12] 刘彦.  滇南小耳猪深Ⅱ度烧(烫)伤模型的建立, 昆明医科大学学报.
    [13] 谢亮焜.  云南省医科类高校学生教学质量满意度调查, 昆明医科大学学报.
    [14] 代冬梅.  沙利度胺治疗皮肤转移性Crohn病1例报道, 昆明医科大学学报.
    [15] 梁刚.  维生素B12滴眼液对青少年近视眼调节的影响, 昆明医科大学学报.
    [16] 梁刚.  维生素B12滴眼液治疗LASIK后出现视疲劳的临床疗效观察, 昆明医科大学学报.
    [17] 李晓非.  噬菌体生物扩增技术在结核分枝杆菌利福平耐药性检测中的应用, 昆明医科大学学报.
    [18] 吴高莉.  噬菌体鉴定食品中沙门菌污染情况调查分析, 昆明医科大学学报.
    [19] 黄芩.  云南部分农村居民对健康相关问题关注度的现况调查, 昆明医科大学学报.
    [20] 柯亭羽.  女性HIV感染患者性满意度的临床调查研究, 昆明医科大学学报.
    • 施引文献
  • 资源附件(0)
  • 加载中
WeChat 点击查看大图
表(4)
计量
  • 文章访问数:  1787
  • HTML全文浏览量:  1560
  • PDF下载量:  32
  • 被引次数: 0
出版历程
  • 收稿日期:  2021-12-15
  • 网络出版日期:  2022-02-24
  • 刊出日期:  2022-03-04

目录

    /

    返回文章
    返回

    版权所有 © 《昆明医科大学学报》编辑部  滇ICP备00000000号-0

    编辑出版:昆明医科大学学报编辑部

    本系统由 北京仁和汇智信息技术有限公司 开发    百度统计