4.7 Article

Efficient manipulation of gene dosage in human iPSCs using CRISPR/Cas9 nickases

COMMUNICATIONS BIOLOGY (2021)

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Journal

COMMUNICATIONS BIOLOGY
Volume 4, Issue 1, Pages -

Publisher

NATURE RESEARCH
DOI: 10.1038/s42003-021-01722-0

Keywords

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Categories

Biology Multidisciplinary Sciences

Funding

  1. National Key R&D Program of China [2017YFE0190000, 2018YFE0203600]
  2. Hong Kong Research Grants Council Theme-based Research Scheme [T13-605/18-W]
  3. Area of Excellence Scheme of the University Grants Committee [AoE/M-604/16]
  4. Innovation and Technology Commission [ITCPD/17-9]
  5. Lee Hysan Foundation [LHF17SC01]
  6. Guangdong Provincial Key ST Program [2018B030336001]
  7. Shenzhen Knowledge Innovation Program [JCYJ20180507183642005, JCYJ20170413165053031, JCYJ20200109115631248, JCYJ20170413173717055]
  8. Shenzhen-Hong Kong Institute of Brain Science-Shenzhen Fundamental Research Institutions [2019SHIBS0001]

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Researchers demonstrate a simple and precise method to simultaneously generate iPSC lines with different gene dosages using paired Cas9 nickases. As proof-of-concept they apply this method to examining amyloid precursor protein gene dosage effects in an Alzheimer's disease patient-derived iPSC line. Their method could potentially advance what we know about disease mechanisms and assist with gene therapy development.
The dysregulation of gene dosage due to duplication or haploinsufficiency is a major cause of autosomal dominant diseases such as Alzheimer's disease. However, there is currently no rapid and efficient method for manipulating gene dosage in a human model system such as human induced pluripotent stem cells (iPSCs). Here, we demonstrate a simple and precise method to simultaneously generate iPSC lines with different gene dosages using paired Cas9 nickases. We first generate a Cas9 nickase variant with broader protospacer-adjacent motif specificity to expand the targetability of double-nicking-mediated genome editing. As a proof-of-concept study, we examine the gene dosage effects on an Alzheimer's disease patient-derived iPSC line that carries three copies of APP (amyloid precursor protein). This method enables the rapid and simultaneous generation of iPSC lines with monoallelic, biallelic, or triallelic knockout of APP. The cortical neurons generated from isogenically corrected iPSCs exhibit gene dosage-dependent correction of disease-associated phenotypes of amyloid-beta secretion and Tau hyperphosphorylation. Thus, the rapid generation of iPSCs with different gene dosages using our method described herein can be a useful model system for investigating disease mechanisms and therapeutic development. Ye et al demonstrate a simple and precise method to simultaneously generate iPSC lines with different gene dosages using paired Cas9 nickases. As proof-of-concept they apply this method to examining amyloid precursor protein gene dosage effects in an Alzheimer's disease patient-derived iPSC line. Their method could potentially advance what we know about disease mechanisms and assist with gene therapy development.

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