Efficient generation of genetically distinct pigs in a single pregnancy using multiplexed single‐guide RNA and carbohydrate selection. (2nd September 2014)
- Record Type:
- Journal Article
- Title:
- Efficient generation of genetically distinct pigs in a single pregnancy using multiplexed single‐guide RNA and carbohydrate selection. (2nd September 2014)
- Main Title:
- Efficient generation of genetically distinct pigs in a single pregnancy using multiplexed single‐guide RNA and carbohydrate selection
- Authors:
- Li, Ping
Estrada, Jose L.
Burlak, Christopher
Montgomery, Jessica
Butler, James R.
Santos, Rafael M.
Wang, Zheng‐Yu
Paris, Leela L.
Blankenship, Ross L.
Downey, Susan M.
Tector, Matthew
Tector, A. Joseph - Abstract:
- <abstract abstract-type="main" id="xen12131-abs-0001"> <title>Abstract</title> <sec id="xen12131-sec-0001" sec-type="section"> <title>Background</title> <p>Manipulating the pig genome to increase compatibility with human biology may facilitate the clinical application of xenotransplantation. Genetic modifications to pig cells have been made by sequential recombination in fetal fibroblasts and liver‐derived cells followed by cross‐breeding or somatic cell nuclear transfer. The generation of pigs for research or organ donation by these methods is slow, expensive and requires technical expertise. A novel system incorporating the bacterial nuclease Cas9 and single‐guide RNA targeting a 20 nucleotide site within a gene can be expressed from a single plasmid leading to a double‐strand break and gene disruption. Coexpression of multiple unique single‐guide RNA can modify several genetic loci in a single step. We describe a process for increasing the efficiency of selecting cells with multiple genetic modifications.</p> </sec> <sec id="xen12131-sec-0002" sec-type="section"> <title>Methods</title> <p>We used the CRISPR/Cas system to target the GGTA1, CMAH and putative iGb3S genes in pigs that have been naturally deleted in humans. Cells lacking galactose α‐1, 3 galactose (α‐Gal) were negatively selected by an IB4 lectin/magnetic bead. α‐Gal negative multiplexed single‐guide RNA‐treated cells were used for somatic cell nuclear transfer (SCNT) and transferred to fertile sows. We<abstract abstract-type="main" id="xen12131-abs-0001"> <title>Abstract</title> <sec id="xen12131-sec-0001" sec-type="section"> <title>Background</title> <p>Manipulating the pig genome to increase compatibility with human biology may facilitate the clinical application of xenotransplantation. Genetic modifications to pig cells have been made by sequential recombination in fetal fibroblasts and liver‐derived cells followed by cross‐breeding or somatic cell nuclear transfer. The generation of pigs for research or organ donation by these methods is slow, expensive and requires technical expertise. A novel system incorporating the bacterial nuclease Cas9 and single‐guide RNA targeting a 20 nucleotide site within a gene can be expressed from a single plasmid leading to a double‐strand break and gene disruption. Coexpression of multiple unique single‐guide RNA can modify several genetic loci in a single step. We describe a process for increasing the efficiency of selecting cells with multiple genetic modifications.</p> </sec> <sec id="xen12131-sec-0002" sec-type="section"> <title>Methods</title> <p>We used the CRISPR/Cas system to target the GGTA1, CMAH and putative iGb3S genes in pigs that have been naturally deleted in humans. Cells lacking galactose α‐1, 3 galactose (α‐Gal) were negatively selected by an IB4 lectin/magnetic bead. α‐Gal negative multiplexed single‐guide RNA‐treated cells were used for somatic cell nuclear transfer (SCNT) and transferred to fertile sows. We examined the levels of α‐Gal and Neu5Gc expression of 32 day fetuses and piglets and analyzed the targeted genes by DNA sequencing.</p> </sec> <sec id="xen12131-sec-0003" sec-type="section"> <title>Results</title> <p>Liver‐derived cells treated with multiple single‐guide RNA and selected for an α‐Gal null phenotype were significantly more likely to also carry mutations in simultaneously targeted genes. Multiplex single‐guide RNA‐treated cells used directly for SCNT without further genetic selection produced piglets with deletions in the targeted genes but also created double‐ and triple‐gene KO variations. CRISPR/Cas‐treated cells grew normally and yielded normal liters of healthy piglets via somatic cell nuclear transfer.</p> </sec> <sec id="xen12131-sec-0004" sec-type="section"> <title>Conclusions</title> <p>The CRISPR/Cas system allows targeting of multiple genes in a single reaction with the potential to create pigs of one genetic strain or multiple genetic modifications in a single pregnancy. The application of this phenotypic selection strategy with multiplexed sgRNA and the Cas9 nuclease has accelerated our ability to produce and evaluate pigs important to xenotransplantation.</p> </sec> </abstract> … (more)
- Is Part Of:
- Xenotransplantation. Volume 22:Number 1(2015:Jan./Feb.)
- Journal:
- Xenotransplantation
- Issue:
- Volume 22:Number 1(2015:Jan./Feb.)
- Issue Display:
- Volume 22, Issue 1 (2015)
- Year:
- 2015
- Volume:
- 22
- Issue:
- 1
- Issue Sort Value:
- 2015-0022-0001-0000
- Page Start:
- 20
- Page End:
- 31
- Publication Date:
- 2014-09-02
- Subjects:
- Xenografts -- Periodicals
Transplantation of organs, tissues, etc -- Periodicals
617.95 - Journal URLs:
- http://onlinelibrary.wiley.com/journal/10.1111/(ISSN)1399-3089 ↗
http://onlinelibrary.wiley.com/ ↗ - DOI:
- 10.1111/xen.12131 ↗
- Languages:
- English
- ISSNs:
- 0908-665X
- Deposit Type:
- Legaldeposit
- View Content:
- Available online (eLD content is only available in our Reading Rooms) ↗
- Physical Locations:
- British Library DSC - 9367.026000
British Library DSC - BLDSS-3PM
British Library STI - ELD Digital store - Ingest File:
- 3515.xml