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A protocol for custom CRISPR Cas9 donor vector construction to truncate genes in mammalian cells using pcDNA3 backbone
BACKGROUND: Clustered regularly interspaced short palindromic repeat (CRISPR) RNA-guided adaptive immune systems are found in prokaryotes to defend cells from foreign DNA. CRISPR Cas9 systems have been modified and employed as genome editing tools in wide ranging organisms. Here, we provide a detail...
| Autores principales: | , , , , , , , , , , , , , , |
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| Formato: | Online Artículo Texto |
| Lenguaje: | English |
| Publicado: |
BioMed Central
2018
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| Materias: | |
| Acceso en línea: | https://www.ncbi.nlm.nih.gov/pmc/articles/PMC5853148/ https://www.ncbi.nlm.nih.gov/pubmed/29540148 http://dx.doi.org/10.1186/s12867-018-0105-8 |
| _version_ | 1783306710976299008 |
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| author | Vazquez, Neftali Sanchez, Lilia Marks, Rebecca Martinez, Eduardo Fanniel, Victor Lopez, Alma Salinas, Andrea Flores, Itzel Hirschmann, Jesse Gilkerson, Robert Schuenzel, Erin Dearth, Robert Halaby, Reginald Innis-Whitehouse, Wendy Keniry, Megan |
| author_facet | Vazquez, Neftali Sanchez, Lilia Marks, Rebecca Martinez, Eduardo Fanniel, Victor Lopez, Alma Salinas, Andrea Flores, Itzel Hirschmann, Jesse Gilkerson, Robert Schuenzel, Erin Dearth, Robert Halaby, Reginald Innis-Whitehouse, Wendy Keniry, Megan |
| author_sort | Vazquez, Neftali |
| collection | PubMed |
| description | BACKGROUND: Clustered regularly interspaced short palindromic repeat (CRISPR) RNA-guided adaptive immune systems are found in prokaryotes to defend cells from foreign DNA. CRISPR Cas9 systems have been modified and employed as genome editing tools in wide ranging organisms. Here, we provide a detailed protocol to truncate genes in mammalian cells using CRISPR Cas9 editing. We describe custom donor vector construction using Gibson assembly with the commonly utilized pcDNA3 vector as the backbone. RESULTS: We describe a step-by-step method to truncate genes of interest in mammalian cell lines using custom-made donor vectors. Our method employs 2 guide RNAs, mutant Cas9D10A nickase (Cas9 = CRISPR associated sequence 9), and a custom-made donor vector for homologous recombination to precisely truncate a gene of interest with a selectable neomycin resistance cassette (NPTII: Neomycin Phosphotransferase II). We provide a detailed protocol on how to design and construct a custom donor vector using Gibson assembly (and the commonly utilized pcDNA3 vector as the backbone) allowing researchers to obtain specific gene modifications of interest (gene truncation, gene deletion, epitope tagging or knock-in mutation). Selection of mutants in mammalian cell lines with G418 (Geneticin) combined with several screening methods: western blot analysis, polymerase chain reaction, and Sanger sequencing resulted in streamlined mutant isolation. Proof of principle experiments were done in several mammalian cell lines. CONCLUSIONS: Here we describe a detailed protocol to employ CRISPR Cas9 genome editing to truncate genes of interest using the commonly employed expression vector pcDNA3 as the backbone for the donor vector. Providing a detailed protocol for custom donor vector design and construction will enable researchers to develop unique genome editing tools. To date, detailed protocols for CRISPR Cas9 custom donor vector construction are limited (Lee et al. in Sci Rep 5:8572, 2015; Ma et al. in Sci Rep 4:4489, 2014). Custom donor vectors are commercially available, but can be expensive. Our goal is to share this protocol to aid researchers in performing genetic investigations that require custom donor vectors for specialized applications (specific gene truncations, knock-in mutations, and epitope tagging applications). ELECTRONIC SUPPLEMENTARY MATERIAL: The online version of this article (10.1186/s12867-018-0105-8) contains supplementary material, which is available to authorized users. |
| format | Online Article Text |
| id | pubmed-5853148 |
| institution | National Center for Biotechnology Information |
| language | English |
| publishDate | 2018 |
| publisher | BioMed Central |
| record_format | MEDLINE/PubMed |
| spelling | pubmed-58531482018-03-22 A protocol for custom CRISPR Cas9 donor vector construction to truncate genes in mammalian cells using pcDNA3 backbone Vazquez, Neftali Sanchez, Lilia Marks, Rebecca Martinez, Eduardo Fanniel, Victor Lopez, Alma Salinas, Andrea Flores, Itzel Hirschmann, Jesse Gilkerson, Robert Schuenzel, Erin Dearth, Robert Halaby, Reginald Innis-Whitehouse, Wendy Keniry, Megan BMC Mol Biol Methodology Article BACKGROUND: Clustered regularly interspaced short palindromic repeat (CRISPR) RNA-guided adaptive immune systems are found in prokaryotes to defend cells from foreign DNA. CRISPR Cas9 systems have been modified and employed as genome editing tools in wide ranging organisms. Here, we provide a detailed protocol to truncate genes in mammalian cells using CRISPR Cas9 editing. We describe custom donor vector construction using Gibson assembly with the commonly utilized pcDNA3 vector as the backbone. RESULTS: We describe a step-by-step method to truncate genes of interest in mammalian cell lines using custom-made donor vectors. Our method employs 2 guide RNAs, mutant Cas9D10A nickase (Cas9 = CRISPR associated sequence 9), and a custom-made donor vector for homologous recombination to precisely truncate a gene of interest with a selectable neomycin resistance cassette (NPTII: Neomycin Phosphotransferase II). We provide a detailed protocol on how to design and construct a custom donor vector using Gibson assembly (and the commonly utilized pcDNA3 vector as the backbone) allowing researchers to obtain specific gene modifications of interest (gene truncation, gene deletion, epitope tagging or knock-in mutation). Selection of mutants in mammalian cell lines with G418 (Geneticin) combined with several screening methods: western blot analysis, polymerase chain reaction, and Sanger sequencing resulted in streamlined mutant isolation. Proof of principle experiments were done in several mammalian cell lines. CONCLUSIONS: Here we describe a detailed protocol to employ CRISPR Cas9 genome editing to truncate genes of interest using the commonly employed expression vector pcDNA3 as the backbone for the donor vector. Providing a detailed protocol for custom donor vector design and construction will enable researchers to develop unique genome editing tools. To date, detailed protocols for CRISPR Cas9 custom donor vector construction are limited (Lee et al. in Sci Rep 5:8572, 2015; Ma et al. in Sci Rep 4:4489, 2014). Custom donor vectors are commercially available, but can be expensive. Our goal is to share this protocol to aid researchers in performing genetic investigations that require custom donor vectors for specialized applications (specific gene truncations, knock-in mutations, and epitope tagging applications). ELECTRONIC SUPPLEMENTARY MATERIAL: The online version of this article (10.1186/s12867-018-0105-8) contains supplementary material, which is available to authorized users. BioMed Central 2018-03-14 /pmc/articles/PMC5853148/ /pubmed/29540148 http://dx.doi.org/10.1186/s12867-018-0105-8 Text en © The Author(s) 2018 Open AccessThis article is distributed under the terms of the Creative Commons Attribution 4.0 International License (http://creativecommons.org/licenses/by/4.0/), which permits unrestricted use, distribution, and reproduction in any medium, provided you give appropriate credit to the original author(s) and the source, provide a link to the Creative Commons license, and indicate if changes were made. The Creative Commons Public Domain Dedication waiver (http://creativecommons.org/publicdomain/zero/1.0/) applies to the data made available in this article, unless otherwise stated. |
| spellingShingle | Methodology Article Vazquez, Neftali Sanchez, Lilia Marks, Rebecca Martinez, Eduardo Fanniel, Victor Lopez, Alma Salinas, Andrea Flores, Itzel Hirschmann, Jesse Gilkerson, Robert Schuenzel, Erin Dearth, Robert Halaby, Reginald Innis-Whitehouse, Wendy Keniry, Megan A protocol for custom CRISPR Cas9 donor vector construction to truncate genes in mammalian cells using pcDNA3 backbone |
| title | A protocol for custom CRISPR Cas9 donor vector construction to truncate genes in mammalian cells using pcDNA3 backbone |
| title_full | A protocol for custom CRISPR Cas9 donor vector construction to truncate genes in mammalian cells using pcDNA3 backbone |
| title_fullStr | A protocol for custom CRISPR Cas9 donor vector construction to truncate genes in mammalian cells using pcDNA3 backbone |
| title_full_unstemmed | A protocol for custom CRISPR Cas9 donor vector construction to truncate genes in mammalian cells using pcDNA3 backbone |
| title_short | A protocol for custom CRISPR Cas9 donor vector construction to truncate genes in mammalian cells using pcDNA3 backbone |
| title_sort | protocol for custom crispr cas9 donor vector construction to truncate genes in mammalian cells using pcdna3 backbone |
| topic | Methodology Article |
| url | https://www.ncbi.nlm.nih.gov/pmc/articles/PMC5853148/ https://www.ncbi.nlm.nih.gov/pubmed/29540148 http://dx.doi.org/10.1186/s12867-018-0105-8 |
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