Abstract
BackgroundHuman importin beta has been used in all Xenopus laevis in vitro nuclear assembly and spindle assembly studies. This disconnect between species raised the question for us as to whether importin beta was an authentic negative regulator of cell cycle events, or a dominant negative regulator due to a difference between the human and Xenopus importin beta sequences. No Xenopus importin beta gene was yet identified at the time of those studies. Thus, we first cloned, identified, and tested the Xenopus importin beta gene to address this important mechanistic difference. If human importin beta is an authentic negative regulator then we would expect human and Xenopus importin beta to have identical negative regulatory effects on nuclear membrane fusion and pore assembly. If human importin beta acts instead as a dominant negative mutant inhibitor, we should then see no inhibitory effect when we added the Xenopus homologue.ResultsWe found that Xenopus importin beta acts identically to its human counterpart. It negatively regulates both nuclear membrane fusion and pore assembly. Human importin beta inhibition was previously found to be reversible by Ran for mitotic spindle assembly and nuclear membrane fusion, but not nuclear pore assembly. During the present study, we observed that this differing reversibility varied depending on the presence or absence of a tag on importin beta. Indeed, when untagged importin beta, either human or Xenopus, was used, inhibition of nuclear pore assembly proved to be Ran-reversible.ConclusionWe conclude that importin beta, human or Xenopus, is an authentic negative regulator of nuclear assembly and, presumably, spindle assembly. A difference in the Ran sensitivity between tagged and untagged importin beta in pore assembly gives us mechanistic insight into nuclear pore formation.
Highlights
Human importin beta has been used in all Xenopus laevis in vitro nuclear assembly and spindle assembly studies
We found Xenopus importin beta to act identically to human importin beta, i.e., it acts as a negative regulator of both nuclear membrane fusion and pore assembly, validating the conclusion that importin beta is an authentic negative regulator of cell cycle steps
Identification and cloning of Xenopus laevis importin beta To address whether human importin beta acts as an authentic negative regulator of nuclear membrane fusion, pore assembly, and spindle assembly, or as a dominant negative mutant inhibitor due to inherent species sequence differences, we set out to identify and clone Xenopus importin beta
Summary
Human importin beta has been used in all Xenopus laevis in vitro nuclear assembly and spindle assembly studies. This disconnect between species raised the question for us as to whether importin beta was an authentic negative regulator of cell cycle events, or a dominant negative regulator due to a difference between the human and Xenopus importin beta sequences. Vertebrate nuclear assembly is a complex process involving the sequential recruitment of specific proteins and membranes to chromatin. The majority of nucleoporins are recruited from soluble cytoplasmic subunits The assembly of these nucleoporins into the 500–1000 protein complex is a daunting task, as nucleoporins must sequentially and precisely assemble in the correct order and location [6,7,8]. Determining the choreographed molecular mechanism by which nucleoporins assemble into functional pores within the double nuclear membranes is a matter of intense research
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