Skip to main content

Lund University Publications

LUND UNIVERSITY LIBRARIES

Genetic substitution of Cdk1 by Cdk2 leads to embryonic lethality and loss of meiotic function of Cdk2

Satyanarayana, Ande ; Berthet, Cyril ; Lopez-Molina, Javier ; Coppola, Vincenzo ; Tessarollo, Lino and Kaldis, Philipp LU orcid (2008) In Development: For advances in developmental biology and stem cells 135(20). p.3389-3400
Abstract

It was believed that Cdk2-cyclin E complexes are essential to drive cells through the G1-S phase transition. However, it was discovered recently that the mitotic kinase Cdk1 (Cdc2a) compensates for the loss of Cdk2. In the present study, we tested whether Cdk2 can compensate for the loss of Cdk1. We generated a knockin mouse in which the Cdk2 cDNA was knocked into the Cdk1 locus (Cdk1Cdk2KI). Substitution of both copies of Cdk1 by Cdk2 led to early embryonic lethality, even though Cdk2 was expressed from the Cdk1 locus. In addition, we generated Cdk2-/- Cdk1+/Cdk2KI mice in which one copy of Cdk2 and one copy of Cdk1 were expressed from the Cdk1 locus and the Cdk2 gene was deleted from the endogenous... (More)

It was believed that Cdk2-cyclin E complexes are essential to drive cells through the G1-S phase transition. However, it was discovered recently that the mitotic kinase Cdk1 (Cdc2a) compensates for the loss of Cdk2. In the present study, we tested whether Cdk2 can compensate for the loss of Cdk1. We generated a knockin mouse in which the Cdk2 cDNA was knocked into the Cdk1 locus (Cdk1Cdk2KI). Substitution of both copies of Cdk1 by Cdk2 led to early embryonic lethality, even though Cdk2 was expressed from the Cdk1 locus. In addition, we generated Cdk2-/- Cdk1+/Cdk2KI mice in which one copy of Cdk2 and one copy of Cdk1 were expressed from the Cdk1 locus and the Cdk2 gene was deleted from the endogenous Cdk2 locus. We found that both male and female Cdk2-/- Cdk1+/Cdk2KI mice were sterile, similar to Cdk2-/- mice, even though they expressed the Cdk2 protein from the Cdk1 locus in testes. The translocational and cell cycle properties of knockin Cdk2 in Cdk2-/- Cdk1+/Cdk2KI cells were comparable to those of endogenous Cdk2, but we detected premature transcriptional activation of Cdk1 during liver regeneration in the absence of Cdk2. This study provides evidence of the molecular differences between Cdk2 and Cdk1 and highlights that the timing of transcriptional activation and the genetic locus play important roles in determining the function of Cdk proteins in vivo.

(Less)
Please use this url to cite or link to this publication:
author
; ; ; ; and
publishing date
type
Contribution to journal
publication status
published
keywords
Cell cyde regulation, Cyclin, Cydin-dependent kinase (Cdk), Meiosis, Mouse genetics
in
Development: For advances in developmental biology and stem cells
volume
135
issue
20
pages
3389 - 3400
publisher
The Company of Biologists Ltd
external identifiers
  • scopus:58149262051
  • pmid:18787066
ISSN
0950-1991
DOI
10.1242/dev.024919
language
English
LU publication?
no
id
cbe816d1-af84-44a4-b5d0-b9a452bc9575
date added to LUP
2019-09-18 14:11:47
date last changed
2025-01-09 23:29:17
@article{cbe816d1-af84-44a4-b5d0-b9a452bc9575,
  abstract     = {{<p>It was believed that Cdk2-cyclin E complexes are essential to drive cells through the G1-S phase transition. However, it was discovered recently that the mitotic kinase Cdk1 (Cdc2a) compensates for the loss of Cdk2. In the present study, we tested whether Cdk2 can compensate for the loss of Cdk1. We generated a knockin mouse in which the Cdk2 cDNA was knocked into the Cdk1 locus (Cdk1<sup>Cdk2KI</sup>). Substitution of both copies of Cdk1 by Cdk2 led to early embryonic lethality, even though Cdk2 was expressed from the Cdk1 locus. In addition, we generated Cdk2<sup>-/-</sup> Cdk1<sup>+/Cdk2KI</sup> mice in which one copy of Cdk2 and one copy of Cdk1 were expressed from the Cdk1 locus and the Cdk2 gene was deleted from the endogenous Cdk2 locus. We found that both male and female Cdk2<sup>-/-</sup> Cdk1<sup>+/Cdk2KI</sup> mice were sterile, similar to Cdk2<sup>-/-</sup> mice, even though they expressed the Cdk2 protein from the Cdk1 locus in testes. The translocational and cell cycle properties of knockin Cdk2 in Cdk2<sup>-/-</sup> Cdk1<sup>+/Cdk2KI</sup> cells were comparable to those of endogenous Cdk2, but we detected premature transcriptional activation of Cdk1 during liver regeneration in the absence of Cdk2. This study provides evidence of the molecular differences between Cdk2 and Cdk1 and highlights that the timing of transcriptional activation and the genetic locus play important roles in determining the function of Cdk proteins in vivo.</p>}},
  author       = {{Satyanarayana, Ande and Berthet, Cyril and Lopez-Molina, Javier and Coppola, Vincenzo and Tessarollo, Lino and Kaldis, Philipp}},
  issn         = {{0950-1991}},
  keywords     = {{Cell cyde regulation; Cyclin; Cydin-dependent kinase (Cdk); Meiosis; Mouse genetics}},
  language     = {{eng}},
  month        = {{12}},
  number       = {{20}},
  pages        = {{3389--3400}},
  publisher    = {{The Company of Biologists Ltd}},
  series       = {{Development: For advances in developmental biology and stem cells}},
  title        = {{Genetic substitution of Cdk1 by Cdk2 leads to embryonic lethality and loss of meiotic function of Cdk2}},
  url          = {{http://dx.doi.org/10.1242/dev.024919}},
  doi          = {{10.1242/dev.024919}},
  volume       = {{135}},
  year         = {{2008}},
}