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. 2004 Winter;9(4):359-68.
doi: 10.1379/csc-29r1.1.

Investigating the protein-protein interactions of the yeast Hsp90 chaperone system by two-hybrid analysis: potential uses and limitations of this approach

Stefan H Millson  1 Andrew W TrumanFrancis WolframVictoria KingBarry PanaretouChrisostomos ProdromouLaurence H PearlPeter W Piper
Affiliations

Investigating the protein-protein interactions of the yeast Hsp90 chaperone system by two-hybrid analysis: potential uses and limitations of this approach

Stefan H Millson et al. Cell Stress Chaperones. 2004 Winter.

Abstract

The Hsp90 chaperone cycle involves sequential assembly of different Hsp90-containing multiprotein complexes, the accessory proteins ("cochaperones") that are associated with these complexes being exchanged as the cycle proceeds from its early to its late stages. To gain insight as to whether the 2-hybrid system could be used to probe the interactions of this Hsp90 system, yeast transformants were constructed that express the Gal4p deoxyribonucleic acid-binding domain (BD) fused to the 2 Hsp90 isoforms and the various Hsp90 system cochaperones of yeast. These "bait" fusions were then introduced by mating into other transformants expressing nearly all the 6000 proteins of yeast expressed as fusions to the Gal4p activation domain (AD). High throughput 2-hybrid screening revealed the ability of Hsp90 and Hsp90 system cochaperones to engage in stable interactions in vivo, both with each other and with the various other proteins of the yeast proteome. Consistent with the transience of most chaperone associations, interactions to Hsp90 itself were invariably weak and generally influenced by stress. Mutations within a Hsp90-BD bait fusion and an AD-Cdc37 "prey" fusion were used to provide in vivo confirmation of the in vitro data that shows that Cdc37p is interacting with the "relaxed" conformation of Hsp90 and also to provide indications that Cdc37p needs to be phosphorylated at its N-terminus for any appreciable interaction with Hsp90. A number of potentially novel cochaperone interactions were also identified, providing a framework for these to be analyzed further using other techniques.

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Figures

Fig 1.
Fig 1.
Phase-contrast images (100× magnification) of representative cells of the hsc82Δ hsp82Δ double mutant (Millson et al 2003) expressing either the wild-type Hsc82 (left) or the Hsc82-BD 2-hybrid bait fusion (right) as the sole form of Hsp90
Fig 2.
Fig 2.
Summary diagram of the Hsp90 (Hsp82) and Hsp90 system cochaperone interactions detected on the basis of HIS3 activation (growth during 10 days in the absence of histidine and the presence of 3-amino-1,2,4-triazole [3-AT]). Baits used (BD fusions) are boxed with a thick line, and their putative interactors (AD-protein fusions) are boxed in thinner lines. Only the interactions detected in 2 separate screens of the array are shown, the thickness of the line denoting the apparent strength of interaction (thin, growth to 1 mM 3-AT; medium, growth to 2 mM 3-AT; thick, growth at 3 mM or higher 3-AT)
Fig 3.
Fig 3.
Stress effects on interactions involving Hsp90 bait fusions. (a) Interactions of Hsp82 with Yol029p and Ylr282p. (b) Interactions of Hsc82 with Yol029p and Ylr282p. (c) Interaction of Hsp82 with Cdc37p. (d) Interaction of Hsp82 with She4p. Cells were either unstressed or stressed for 1 hour under the conditions detailed in Methods. Because the low basal expression of the GAL7 promoter-regulated LacZ gene in this system is generally due to the AD-protein fusion, LacZ expression values are in all cases expressed relative to the control PJ69-4 cells containing the plasmid for expression of this AD-fusion and empty pBDC. Control experiments showed that the interaction signal for the Hsp82-BD or Hsc82-BD “bait” fusion plus empty AD vector was unaffected by all these stress treatments (mean and standard deviation in 4 separate experiments being 1.8 ± 0.3, 2.1 ± 0.3, 2.1 ± 0.5, and 1.5 ± 0.4 units of β-galactosidase per 1 × 106 cells for the unstressed, heat shocked, sorbitol-treated, and heat shocked plus sorbitol-treated samples, respectively)
Fig 4.
Fig 4.
The effects of mutations in the Hsp82-BD “bait” or AD-Cdc37p “prey” fusions on the strength of Hsp82-BD–AD-Cdc37p interaction, measured at 22°C (relative to LacZ expression values of the control PJ69-4 cells containing empty pBDC and the plasmid for expression of the corresponding AD-Cdc37p fusion)
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References

    1. Abbas-Terki T, Donze O, Briand PA, Picard D. Hsp104 interacts with hsp90 cochaperones in respiring yeast. Mol Cell Biol. 2001;21:7569–7575.0270-7306(2001)021<7569:HIWHCI>2.0.CO;2 - PMC - PubMed
    1. Adams A, Gottschling DE, Kaiser CA, and Stearns T 1997 Methods in Yeast Genetics. Cold Spring Harbor Laboratory Press, Cold Spring Harbor, NY.
    1. Bandhakavi S, McCann RO, Hanna DE, Glover CV. A positive feedback loop between protein kinase CKII and Cdc37 promotes the activity of multiple protein kinases. J Biol Chem. 2003;278:2829–2836.0021-9258(2003)278<2829:APFLBP>2.0.CO;2 - PubMed
    1. Barral JM, Hutagalung AH, Brinker A, Hartl FU, Epstein HF. Role of the myosin assembly protein UNC-45 as a molecular chaperone for myosin. Science. 2002;295:669–771.0193-4511(2002)295<0669:ROTMAP>2.0.CO;2 - PubMed
    1. Bohen SP. Genetic and biochemical analysis of p23 and ansamycin antibiotics in the function of Hsp90-dependent signaling proteins. Mol Cell Biol. 1998;18:3330–3339.0270-7306(1998)018<3330:GABAOP>2.0.CO;2 - PMC - PubMed

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