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Literature DB >> 7565735

Correlation of two-hybrid affinity data with in vitro measurements.

Abstract

Since their introduction, the interaction trap and other two-hybrid systems have been used to study protein-protein interactions. Despite their general use, little is known about the extent to which the degree of protein interaction determined by two-hybrid approaches parallels the degree of interaction determined by biochemical techniques. In this study, we used a set of lexAop-LEU2 and lexAop-lacZ reporters to calibrate the interaction trap. For the calibration, we used two sets of proteins, the Myc-Max-Mxi1 helix-loop-helix proteins, and wild-type and dimerization-defective versions of the lambda cI repressor. Our results indicate that the strength of interaction as predicted by the two-hybrid approach generally correlates with that determined in vitro, permitting discrimination of high-, intermediate-, and low-affinity interactions, but there was no single reporter for which the amount of gene expression linearly reflected affinity measured in vitro. However, some reporters showed thresholds and only responded to stronger interactions. Finally, some interactions were subject to directionality, and their apparent strength depended on the reporter used. Taken together, our results provide a cautionary framework for interpreting affinities from two-hybrid experiments.

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Year: 1995 PMID： 7565735 PMCID： PMC230834 DOI： 10.1128/MCB.15.10.5820

Source DB: PubMed Journal: Mol Cell Biol ISSN： 0270-7306 Impact factor: 4.272

47 in total

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Journal: Science Date: 1976-10-08 Impact factor: 47.728

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Authors: Y Ebina; Y Takahara; F Kishi; A Nakazawa; R Brent
Journal: J Biol Chem Date: 1983-11-10 Impact factor: 5.157

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Authors: R Brent; M Ptashne
Journal: Nature Date: 1984 Dec 13-19 Impact factor: 49.962

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Authors: S Cohen; B J Knoll; J W Little; D W Mount
Journal: Nature Date: 1981-11-12 Impact factor: 49.962

6. Mechanism of action of the lexA gene product.

Authors: R Brent; M Ptashne
Journal: Proc Natl Acad Sci U S A Date: 1981-07 Impact factor: 11.205

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Authors: A Laughon; R F Gesteland
Journal: Proc Natl Acad Sci U S A Date: 1982-11 Impact factor: 11.205

8. A eukaryotic transcriptional activator bearing the DNA specificity of a prokaryotic repressor.

Authors: R Brent; M Ptashne
Journal: Cell Date: 1985-12 Impact factor: 41.582

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Authors: H Ito; Y Fukuda; K Murata; A Kimura
Journal: J Bacteriol Date: 1983-01 Impact factor: 3.490

10. Saccharomyces cerevisiae GAL1-GAL10 divergent promoter region: location and function of the upstream activating sequence UASG.

Authors: R W West; R R Yocum; M Ptashne
Journal: Mol Cell Biol Date: 1984-11 Impact factor: 4.272

185 in total

Correlation of two-hybrid affinity data with in vitro measurements.

1. Autoregulation and function of a repressor in bacteriophage lambda.

2. The lambda repressor contains two domains.

3. LexA protein is a repressor of the colicin E1 gene.

4. A bacterial repressor protein or a yeast transcriptional terminator can block upstream activation of a yeast gene.

5. Preferential cleavage of phage lambda repressor monomers by recA protease.

6. Mechanism of action of the lexA gene product.

7. Isolation and preliminary characterization of the GAL4 gene, a positive regulator of transcription in yeast.

8. A eukaryotic transcriptional activator bearing the DNA specificity of a prokaryotic repressor.

9. Transformation of intact yeast cells treated with alkali cations.

10. Saccharomyces cerevisiae GAL1-GAL10 divergent promoter region: location and function of the upstream activating sequence UASG.

1. The zinc finger-associated SCAN box is a conserved oligomerization domain.

2. A cell plate-specific callose synthase and its interaction with phragmoplastin.

3. "Mutagenesis" by peptide aptamers identifies genetic network members and pathway connections.

4. Searching interaction partners of protein kinase CK2beta subunit by two-hybrid screening.

5. Targeted modification and transportation of cellular proteins.

6. COP I domains required for coatomer integrity, and novel interactions with ARF and ARF-GAP.

7. Interaction of the repressors Nrg1 and Nrg2 with the Snf1 protein kinase in Saccharomyces cerevisiae.

8. Detection of peptides, proteins, and drugs that selectively interact with protein targets.

9. Interaction of recombinant myocilin with the matricellular protein SPARC: functional implications.

10. Characterization and expression of a rice RAD23 gene.