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Nuclear transport of plant potyviral proteins.

Maria A. Restrepo, +2 more
- 01 Oct 1990 - 
- Vol. 2, Iss: 10, pp 987-998
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TLDR
The results indicate that both Nla and Nlb contain nuclear targeting signals, and that they may serve as useful models for studies of plant cell nuclear transport.
Abstract
We have used immunoblotting, immunocytochemical, and gene fusion methods to examine the differential subcellular partitioning of tobacco etch potyvirus proteins that are potentially associated with RNA replication. From the earliest timepoints at which viral proteins could be detected, proteins Nla (49-kilodalton proteinase) and Nlb (58-kilodalton polymerase) were localized primarily in the nucleus, whereas the 71-kilodalton cylindrical inclusion protein was identified in the cytoplasm. The Nla and Nlb coding regions were fused to the beta-glucuronidase (GUS) sequence in a plant expression vector, resulting in synthesis of chimeric proteins in transfected protoplasts and in transgenic plants. In situ localization of GUS activity revealed nuclear localization of the GUS-Nla and GUS-Nlb fusion proteins and cytoplasmic localization of nonfused GUS. These results indicate that both Nla and Nlb contain nuclear targeting signals, and that they may serve as useful models for studies of plant cell nuclear transport. A discussion of the general utility of the nuclear transport system described here, as well as the role of nuclear translocation of potyviral proteins, is presented.

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P1/HC-Pro, a Viral Suppressor of RNA Silencing, Interferes with Arabidopsis Development and miRNA Function

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Activation of the ethylene gas response pathway in Arabidopsis by the nuclear protein ETHYLENE-INSENSITIVE3 and related proteins.

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Arabidopsis WRKY33 transcription factor is required for resistance to necrotrophic fungal pathogens

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PIF3, a phytochrome-interacting factor necessary for normal photoinduced signal transduction, is a novel basic helix-loop-helix protein.

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A mutation in Arabidopsis that leads to constitutive expression of systemic acquired resistance.

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References
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Journal ArticleDOI

Assaying chimeric genes in plants: The GUS gene fusion system

TL;DR: Gene fusions can be defined its DNA constructions that result in the coding sequences from one gene (r@o,ter) being transcribed and/or translated under the direction of the controlling sequences of another gene (cmltrr).
Journal ArticleDOI

The rapid generation of oligonucleotide-directed mutations at high frequency using phosphorothioate-modified DNA

TL;DR: Two methods are described by which this approach has been used to produce mutations in M13mp2 phage DNA with high efficiency as a result of simple and rapid in vitro manipulations.
Journal ArticleDOI

Multiple mechanisms of protein insertion into and across membranes.

TL;DR: Differences in the timing of protein synthesis and translocation into or across the bilayer and in the requirement for a transmembrane electrochemical potential are compared.
Journal ArticleDOI

Hybrid genes in the analysis of transformation conditions : I. Setting up a simple method for direct gene transfer in plant protoplasts.

TL;DR: This paper analyses numerous transformation parameters in a comparative study on SR1Nicotiana tabacum and N. plumbaginifolia, and reports on a simple chemical technique for very efficient protoplast transformation based on the synergistic interaction of MgCl2 and PEG.
Journal ArticleDOI

Nuclear protein migration involves two steps: rapid binding at the nuclear envelope followed by slower translocation through nuclear pores.

TL;DR: This work proposes two steps in nuclear migration of proteins: rapid binding around the nuclear envelope, possibly to pore-associated fibrils, followed by slower, energy-dependent translocation through nuclear pores.
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