CRISPR-on for activation of endogenous SMARCA4 and TFAP2C expression in bovine embryos

Author:

Savy Virginia1,Alberio Virgilia1,Canel Natalia G1,Ratner Laura D1,Gismondi Maria I2,Ferraris Sergio F3,Fernandez-Martín Rafael1,Knott Jason G4,Bevacqua Romina J15,Salamone Daniel F1

Affiliation:

1. 1Laboratorio de Biotecnología Animal, Facultad de Agronomía, Universidad de Buenos Aires/INPA CONICET, CABA, Argentina

2. 2Instituto de Biotecnología, CICVyA, INTA, Hurlingam, Buenos Aires, Argentina

3. 3Centro de Ciencias Veterinarias, Universidad Maimónides, CABA, Argentina

4. 4Department of Animal Science, Michigan State University, East Lansing, Michigan, USA

5. 5Seung Kim Lab, Department of Developmental Biology, Stanford University School of Medicine, Stanford, California, USA

Abstract

CRISPR-mediated transcriptional activation, also known as CRISPR-on, has proven efficient for activation of individual or multiple endogenous gene expression in cultured cells from several species. However, the potential of CRISPR-on technology in preimplantation mammalian embryos remains to be explored. Here, we report for the first time the successful modulation of endogenous gene expression in bovine embryos by using the CRISPR-on system. As a proof of principle, we targeted the promoter region of either SMARCA4 or TFAP2C genes, transcription factors implicated in trophoblast lineage commitment during embryo development. We demonstrate that CRISPR-on provides temporal control of endogenous gene expression in bovine embryos, by simple cytoplasmic injection of CRISPR RNA components into one cell embryos. dCas9VP160 activator was efficiently delivered and accurately translated into protein, being detected in the nucleus of all microinjected blastomeres. Our approach resulted in the activation of SMARCA expression shortly after microinjection, with a consequent effect on downstream differentiation promoting factors, such as TFAP2C and CDX2. Although targeting of TFAP2C gene did not result in a significant increase in TFAP2C expression, there was a profound induction in CDX2 expression on day 2 of development. Finally, we demonstrate that CRISPR-on system is suitable for gene expression modulation during the preimplantation period, since no detrimental effect was observed on microinjected embryo development. This study constitutes a first step toward the application of the CRISPR-on system for the study of early embryo cell fate decisions in cattle and other mammalian embryos, as well as to design novel strategies that may lead to an improved trophectoderm development.

Publisher

Bioscientifica

Subject

Cell Biology,Obstetrics and Gynecology,Endocrinology,Embryology,Reproductive Medicine

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