园艺学报 ›› 2022, Vol. 49 ›› Issue (7): 1532-1544.doi: 10.16420/j.issn.0513-353x.2021-0475
左鑫1, 李铭铭1, 李欣容1, 苗春妍1, 李炎枋1, 杨旭1, 张重义2, 王丰青1,*()
收稿日期:
2021-11-15
修回日期:
2022-03-15
出版日期:
2022-07-25
发布日期:
2022-07-29
通讯作者:
王丰青
E-mail:heauzycxw@126.com
基金资助:
ZUO Xin1, LI Mingming1, LI Xinrong1, MIAO Chunyan1, LI Yanfang1, YANG Xu1, ZHANG Zhongyi2, WANG Fengqing1,*()
Received:
2021-11-15
Revised:
2022-03-15
Online:
2022-07-25
Published:
2022-07-29
Contact:
WANG Fengqing
E-mail:heauzycxw@126.com
摘要:
为了研究CRISPR/Cas9技术在天目地黄基因编辑中的应用,克隆了天目地黄(Rehmannia chingii)的八氢番茄红素脱氢酶基因(RcPDS1),利用PCR方法扩增其cDNA序列和基因组DNA序列。通过构建单靶点CRISPR/Cas9载体,利用根癌农杆菌介导的遗传转化方法侵染天目地黄无菌苗叶盘,通过TA克隆测序法分析基因编辑的类型。结果显示,克隆获得了1个天目地黄RcPDS1的全长cDNA序列,其具有1个长度为1 743 bp的开放阅读框,编码580个氨基酸残基,基因组DNA序列长度8 041 bp,包含14个内含子和15个外显子。通过遗传转化共获得57个转基因再生株系,其中具明显白化表型的株系有20个(35.09%)。TA克隆测序结果显示,RcPDS1靶位点突变类型主要包括碱基缺失、替换和插入。利用CRISPR/Cas9基因编辑技术在天目地黄中成功实现了对RcPDS1基因的靶向敲除。
中图分类号:
左鑫, 李铭铭, 李欣容, 苗春妍, 李炎枋, 杨旭, 张重义, 王丰青. CRISPR/Cas9技术在天目地黄RcPDS1基因编辑中的应用[J]. 园艺学报, 2022, 49(7): 1532-1544.
ZUO Xin, LI Mingming, LI Xinrong, MIAO Chunyan, LI Yanfang, YANG Xu, ZHANG Zhongyi, WANG Fengqing. CRISPR/Cas9 Technology for RcPDS1 Gene Editing in Rehmannia chingii[J]. Acta Horticulturae Sinica, 2022, 49(7): 1532-1544.
用途 Aim | 产物长度/bp Product size | 引物名称 Primer name | 引物序列(5′-3′) Primer sequence |
---|---|---|---|
RcPDS1扩增 Amplification of RcPDS1 | 6 781(DNA) 1 882(cDNA) | RcPDS1_F | CAGTTGCCTGAGCTGTTGAA |
RcPDS1_R | GCTTCCCTATCTTCTGTCTTCC | ||
RcPDS1 qRT-PCR | 103 | RcPDS1_qF | TATCATTTGCAGTTAGTG |
RcPDS1_qR | ACAACTTTCAAAGGGATTGC | ||
靶序列的合成 Construction of target site | 19 | sgRcPDS1_F | AAGCAAGGGATGTGCTGGG |
sgRcPDS1_R | CCCAGCACATCCCTTGCTT | ||
转基因鉴定 Identification of the transformation | 474 | Cas9_F | TCAACGGCATTCGGGACAAG |
Cas9_R | CCACATACATATCGCGGCCA | ||
281 | pKSE401_F | TGTCCCAGGATTAGAATGATTAGGC | |
sgRcPDS1_R | CCCAGCACATCCCTTGCTT | ||
靶位点序列扩增 Amplification of target region | 1 387 | RcPDS1_TF | CTTCTCCTCGTCCAAACAAG |
RcPDS1_TR | AGCTCTCCAAACAGGTTCTG | ||
Gap序列扩增 Amplification of the gap sequence | 828 | PDSgap1_F | CAGCGAAAACAAGCTGAATCTG |
PDSgap1_R | GATTTCCTCCAAACTAACCGTG | ||
PDSgap2_F | TCGGACATGTTTCTGCTATCAA | ||
2 091 | PDSgap2_R | TCCTTCCATTGCAACCGATC | |
1 012 | PDSgap3_F | ACAAACCAGGAGAGTTCAGC | |
PDSgap3_R | GCTTCAACATAAGACTGACCG | ||
278 | PDSgap4_F | CCTGGTACCGAACCTTGTC | |
RcPDS1_R | GCTTCCCTATCTTCTGTCTTCC |
表1 引物名称及序列
Table 1 Primer names and sequences
用途 Aim | 产物长度/bp Product size | 引物名称 Primer name | 引物序列(5′-3′) Primer sequence |
---|---|---|---|
RcPDS1扩增 Amplification of RcPDS1 | 6 781(DNA) 1 882(cDNA) | RcPDS1_F | CAGTTGCCTGAGCTGTTGAA |
RcPDS1_R | GCTTCCCTATCTTCTGTCTTCC | ||
RcPDS1 qRT-PCR | 103 | RcPDS1_qF | TATCATTTGCAGTTAGTG |
RcPDS1_qR | ACAACTTTCAAAGGGATTGC | ||
靶序列的合成 Construction of target site | 19 | sgRcPDS1_F | AAGCAAGGGATGTGCTGGG |
sgRcPDS1_R | CCCAGCACATCCCTTGCTT | ||
转基因鉴定 Identification of the transformation | 474 | Cas9_F | TCAACGGCATTCGGGACAAG |
Cas9_R | CCACATACATATCGCGGCCA | ||
281 | pKSE401_F | TGTCCCAGGATTAGAATGATTAGGC | |
sgRcPDS1_R | CCCAGCACATCCCTTGCTT | ||
靶位点序列扩增 Amplification of target region | 1 387 | RcPDS1_TF | CTTCTCCTCGTCCAAACAAG |
RcPDS1_TR | AGCTCTCCAAACAGGTTCTG | ||
Gap序列扩增 Amplification of the gap sequence | 828 | PDSgap1_F | CAGCGAAAACAAGCTGAATCTG |
PDSgap1_R | GATTTCCTCCAAACTAACCGTG | ||
PDSgap2_F | TCGGACATGTTTCTGCTATCAA | ||
2 091 | PDSgap2_R | TCCTTCCATTGCAACCGATC | |
1 012 | PDSgap3_F | ACAAACCAGGAGAGTTCAGC | |
PDSgap3_R | GCTTCAACATAAGACTGACCG | ||
278 | PDSgap4_F | CCTGGTACCGAACCTTGTC | |
RcPDS1_R | GCTTCCCTATCTTCTGTCTTCC |
图5 CRISPR/Cas9靶位点选择与重组质粒的构建A:RcPDS1基因及靶点设计;B:PCR鉴定结果;C:重组质粒结构。
Fig. 5 CRISPR/Cas9 target site selection and recombinant plasmid constructionA:Schematic diagram showing RcPDS1 gene structure;B:Result of transformation detection by PCR;C:Schematic of the CRISPR/Cas9 binary vector pKSE401.
图6 天目地黄遗传转化与白化表型突变体A:抗性筛选;B:抗性白化愈伤组织;C:抗性白化芽再生;D:白化芽与绿芽共生;E:白化苗在光照下生长;F:褐化的白化苗;G:完全白化的分化芽;H:白绿嵌合苗。
Fig. 6 Genetic transformation of Rehmannia chingii and albino phenotype mutantsA:Embryogenic calluses were cultured on the medium with kanamycine;B:Positive albino callus;C:Positive albino shoot;D:Positive albino shoot and green shoot regenerated from the same callus;E:Positive albino shoot cultured under light;F:Browning albino shoots;G:Fully albino shoot;H:Chimeric albino shoot.
图9 天目地黄转基因植株RcPDS1靶点突变绿色字母为插入碱基,粉红色字母为替换碱基,短横线为缺失碱基,右边数字为变异碱基 × 克隆数。
Fig. 9 RcPDS1 target mutations in transgenic plants of Rehmannia chingiiGreen letters are insertions,pink letters are substitutions,dashes are deletions,and the number at the right-hand side represent types of base mutation.
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