doi: 10.1091/mbc.e02-11-0708.
Epub 2003 Feb 21.
Genetic evidence for a role of BiP/Kar2 that regulates Ire1 in response to accumulation of unfolded proteins
Affiliations
- PMID: 12808051
- PMCID: PMC194903
- DOI: 10.1091/mbc.e02-11-0708
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Genetic evidence for a role of BiP/Kar2 that regulates Ire1 in response to accumulation of unfolded proteins
Mol Biol Cell.
2003 Jun.
Abstract
In the unfolded protein response (UPR) signaling pathway, accumulation of unfolded proteins in the endoplasmic reticulum (ER) activates a transmembrane kinase/ribonuclease Ire1, which causes the transcriptional induction of ER-resident chaperones, including BiP/Kar2. It was previously hypothesized that BiP/Kar2 plays a direct role in the signaling mechanism. In this model, association of BiP/Kar2 with Ire1 represses the UPR pathway while under conditions of ER stress, BiP/Kar2 dissociation leads to activation. To test this model, we analyzed five temperature-sensitive alleles of the yeast KAR2 gene. When cells carrying a mutation in the Kar2 substrate-binding domain were incubated at the restrictive temperature, association of Kar2 to Ire1 was disrupted, and the UPR pathway was activated even in the absence of extrinsic ER stress. Conversely, cells carrying a mutation in the Kar2 ATPase domain, in which Kar2 poorly dissociated from Ire1 even in the presence of tunicamycin, a potent inducer of ER stress, were unable to activate the pathway. Our findings provide strong evidence in support of BiP/Kar2-dependent Ire1 regulation model and suggest that Ire1 associates with Kar2 as a chaperone substrate. We speculate that recognition of unfolded proteins is based on their competition with Ire1 for binding with BiP/Kar2.
Figures
Schematic representation of the Kar2 protein and kar2 mutant
alleles used in this study. Based on the sites of mutation, kar2
mutant alleles were categorized either as ATPase domain mutants (type A) or
substrate-binding domain mutants (type S).
Altered UPR in kar2 mutant strains. (A) Cells transformed with the
UPRE-lacZ reporter plasmid pCZY1 were exponentially grown to an
OD600 of 0.3 at 23°C in SC medium, and at time (t =
0), the cultures were shifted to 37°C. Tunicamycin was added to a final
concentration of 0 μg/ml (TM -)or2 μg/ml (TM +) at 3 min, and the
cultures were subjected to a β-galactosidase assay at 200 min. Data
presented are the averages of three independent transformants with SD as
indicated by error bars. (B) Cells transformed with pCZY1 were exponentially
grown to an OD600 of 0.2 at 23°C in SD medium, and at time
(t = 0), the cultures were shifted to 37°C (indicated as
37°C) or further cultured at 23°C (indicated as 23°C). Tunicamycin
was added to a final concentration of 0 μg/ml (TM -)or 2 μg/ml (TM +) at
3 min, and the cultures were subjected to β-galactosidase assay at 200
min. Data are presented as described in the legend to the A. (C) Cells were
exponentially grown to an OD600 of 0.4 at 23°C in YPD medium,
and at time (t = 0), the cultures were shifted to 37°C.
Tunicamycin was added to a final concentration of 0 μg/ml (TM -)or 2
μg/ml (TM +) at 3 min, and the cells were collected at 60 min to extract
total cellular RNA for Northern blot analysis using the HAC1 DNA
probe. (D) Percentages of HAC1 mRNA cleavage in C were calculated as
described in MATERIAL AND METHODS.
Altered association or dissociation of Kar2 with Ire1 in kar2
mutant strains. The indicated strains transformed with the Ire1-HA expression
plasmid pRS426-Ire1HA (lanes 2–15), or MS10 cells containing an empty
vector pRS426 (lane 1) were exponentially grown to an OD600 of 0.4
at 23°C in SC medium. At time (t = 0), the cultures were shifted
to 37°C. Tunicamycin was added to a final concentration of 0 μg/ml (TM
-) or 2 μg/ml (TM +) at 3 min, and cells were collected at 60 min to
prepare their lysates (In lane 1, no tunicamycin was added). Anti-HA
immunoprecipitates equivalent to 1 × 108 cells for the lowest
panel, and lysates or anti-HA immunoprecipitates equivalent to 1 ×
107 cells for the other panels were fractionated by 8% SDS-PAGE.
Proteins were detected by subsequent Western blotting with the indicated
antibodies. After treatment with ECL chemiluminescence reagents, the blots
were exposed to x-ray films for the following times: 10 s for the lowest panel
and 2 s for the other panels.
Impaired coaggregation of Kar2 with a model unfolded protein in
kar2 type S mutant strains. Cells transformed with the Δpro
expression plasmid pYPR3841U or an empty vector pRS426 were exponentially
grown to an OD600 of 0.2 at 23°C in SCG medium, and the
cultures were shifted to 37°C (or 34°C for the kar2-133
strain) for 60 min. Cell lysates were prepared from the resulting cultures and
ultracentrifuged at 100,000 × g for 15 min, and the supernatant
and pellet fractions were collected (A and B). (A) Supernatant (S) and pellet
(P) fractions (equivalent to 1 × 107 cells) prepared from
cells containing pYPR3841U were analyzed by anti-RNAP1 Western blotting. (B)
Supernatant (S; equivalent to 1 × 107 cells) and pellet (P;
equivalent to 5 × 107 cells) fractions prepared from cells
containing pYPR3841U (Δpro +) or pRS426 (Δpro -) were analyzed by
anti-Kar2 Western blotting. The asterisk indicates a nonspecific band. In both
panels A and B, the blots treated with ECL reagent were exposed to x-ray films
for 2 s. (C) Lysates from W303 cells carrying pYPR3841U were treated with
control DMSO or 2 mM DSP and ultracentrifuged. The resulting pellet fraction
(input) were dissolved in 1% SDS, and subjected to immunoprecipitation with
anti-Kar2 antiserum or control preimmune serum. The inputs (equivalent to 1
× 107 cells for the upper panel or 3 × 107
cells for the lower panel) or immunoprecipitates (equivalent to 3 ×
107 cells for the upper panel or 9 × 107 cells for
the lower panel) were analyzed by reducing SDS-PAGE followed by anti-Kar2 and
anti-RNAP Western blotting.
Induction of the KAR2 gene in kar2 mutants results
partially from activation of the heat shock response pathway. (A) Cells were
exponentially grown to an OD600 of 0.4 at 23°C in YPD medium,
and shifted to 37°C (37°C) or further cultured at 23°C (23°C)
for 60 min. The resulting cells were used to extract total cellular RNA for
Northern blot analysis using the KAR2, SSA1, and ACT1 DNA
probes. (B) The RNAs shown in A were quantitated and normalized to
ACT1 mRNA. Normalized mRNA values are presented relative to their
levels of expression in MS10 cells cultured at 23°C. (C) Cells transformed
with the HSE-lacZ reporter plasmid pKAR2HSE-lacZ were exponentially
grown to an OD600 of 0.3 at 23°C in SC medium and shifted to 37°C for
200 min, followed by β-galactosidase assay. For an unknown reason, this
HSE-lacZ reporter did not work in the W303 background strains.
A schematic model to interpret our present observations. See text for
explanation.
References
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