Engineering the ribosomal DNA in a megabase synthetic chromosome.

نویسندگان

  • Weimin Zhang
  • Guanghou Zhao
  • Zhouqing Luo
  • Yicong Lin
  • Lihui Wang
  • Yakun Guo
  • Ann Wang
  • Shuangying Jiang
  • Qingwen Jiang
  • Jianhui Gong
  • Yun Wang
  • Sha Hou
  • Jing Huang
  • Tianyi Li
  • Yiran Qin
  • Junkai Dong
  • Qin Qin
  • Jiaying Zhang
  • Xinzhi Zou
  • Xi He
  • Li Zhao
  • Yibo Xiao
  • Meng Xu
  • Erchao Cheng
  • Ning Huang
  • Tong Zhou
  • Yue Shen
  • Roy Walker
  • Yisha Luo
  • Zheng Kuang
  • Leslie A Mitchell
  • Kun Yang
  • Sarah M Richardson
  • Yi Wu
  • Bing-Zhi Li
  • Ying-Jin Yuan
  • Huanming Yang
  • Jiwei Lin
  • Guo-Qiang Chen
  • Qingyu Wu
  • Joel S Bader
  • Yizhi Cai
  • Jef D Boeke
  • Junbiao Dai
چکیده

We designed and synthesized a 976,067-base pair linear chromosome, synXII, based on native chromosome XII in Saccharomyces cerevisiae SynXII was assembled using a two-step method, specified by successive megachunk integration and meiotic recombination-mediated assembly, producing a functional chromosome in S. cerevisiae. Minor growth defect "bugs" detected in synXII, caused by deletion of tRNA genes, were rescued by introducing an ectopic copy of a single tRNA gene. The ribosomal gene cluster (rDNA) on synXII was left intact during the assembly process and subsequently replaced by a modified rDNA unit used to regenerate rDNA at three distinct chromosomal locations. The signature sequences within rDNA, which can be used to determine species identity, were swapped to generate a Saccharomyces synXII strain that would be identified as Saccharomyces bayanus by standard DNA barcoding procedures.

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عنوان ژورنال:
  • Science

دوره 355 6329  شماره 

صفحات  -

تاریخ انتشار 2017