Spatial quality control bypasses cell-based limitations on proteostasis to promote prion curing

  1. Courtney L Klaips
  2. Megan L Hochstrasser
  3. Christine R Langlois
  4. Tricia R Serio  Is a corresponding author
  1. Brown University, United States
  2. University of Arizona, United States
8 figures and 4 tables

Figures

Figure 1 with 1 supplement
Thermal stress induces curing through resolution of Sup35 amyloid.

(A) [PSI+]Strong (SLL2606) and [PSI+]Weak (SLL2600) cultures were incubated for 30 min at the indicated temperatures before plating on rich medium at 30°C to analyze curing by colony color phenotype, as described in the text. (B) Quantification of [PSI+]Weak (SLL2600) colony color phenotypes following treatment as described in (A). Colonies were scored as completely [psi] (black), or sectored (partially [psi], white). Data represent averages; error bars represent standard deviations; n = 3. (C) Semi-native lysates of [psi] (SLL2119), [PSI+]Weak (SLL2600), and [PSI+]Strong (SLL2606) cultures were analyzed by semi-denaturing detergent agarose gel electrophoresis (SDD-AGE) and immunoblotting for Sup35 after treatment as described in (A). (D) Sup35 released from amyoid aggregates in a [PSI+]Weak strain (SLL2600) following treatment as described in (A) and recovery at 30°C in the presence of cycloheximide was determined by treating lysates with 2% SDS at 53°C, followed by SDS-PAGE and quantitative immunoblotting for Sup35. Lines represent medians; boxes represents upper and lower quartiles, and whiskers represent maximum and minimum; n = 5; *p = 0.02, **p = 0.01 by paired t-test.

https://doi.org/10.7554/eLife.04288.003
Figure 1—figure supplement 1
Characterization of thermal stress effects.

(A). Exponentially growing [PSI+]Weak cultures (SLL2600) were incubated at 30°C, 37°C, 40°C, or 37°C before 40°C for 30 min and plated to YPD at 30°C to quantify colony forming units. Data represent means; error bars represent standard deviations; n ≥ 3. (B) [PSI+]Weak cultures (SLL2600) grown exponentially for 2 hr after dilution from a saturated overnight culture (left) or for at least 24 hr (right) were incubated at 40°C for 30 min and allowed to recover for 2 hr at 30°C. Lysates isolated from these cultures were analyzed by SDD-AGE and immunoblotting for Sup35.

https://doi.org/10.7554/eLife.04288.004
Curing is mediated by Hsp104 and depends upon propagation efficiency.

(A) [PSI+]Weak cultures (SLL2600) were incubated at 40°C for 30 min in the absence (untreated) or presence of guanidine HCl (GdnHCl) and plated on YPD to quantify prion loss by colony color phenotype. Data represent means; error bars represent standard deviations; n = 3; p = 0.0004 by unpaired t-test. (B) A WT (HSP104/+; SY945) and a heterozygous disruption (HSP104/Δ; SY591) [PSI+]Weak diploid strain were incubated at 40°C for 90 min and plated on YPD to quantify prion loss by colony color phenotype. Data represent means; error bars represent standard deviations; n = 3; p < 0.0001 by unpaired t-test. (C) [PSI+]Strong strains expressing an extra copy of either WT (SY1646) or G58D (SY1648) Sup35 were incubated at 40°C for 90 min and plated on YPD to quantify prion loss by colony color phenotype. Data represent means; error bars represent standard deviations; n = 4; p < 0.0001 by unpaired t-test. (D) A WT (SUP35/+; SLL3071) and a heterozygous disruption (SUP35/Δ; SY957) diploid [PSI+]Strong strain were incubated at 40°C for 90 min and plated on YPD to quantify prion loss by colony color phenotype. Data represent means; error bars represent standard deviations; n = 3; p < 0.0001 by unpaired t-test.

https://doi.org/10.7554/eLife.04288.005
Figure 3 with 1 supplement
Heat-induced aggregate accumulation but not chaperone levels correlate with temperature.

(A) A [PSI+]Weak strain (SLL2600) was incubated at 30°C, 37°C, 40°C, or 37°C before 40°C for 30 min, and lysates were prepared and analyzed by SDS-PAGE and quantitative immunoblotting for Hsp104 (black), Ssa1 (gray), and Sis1 (white). Data represent means; error bars represent standard deviations; n ≥ 3. (B) Aggregates from lysates of a [PSI+]Weak strain (SLL2600) following treatment as described in (A) were prepared and analyzed by differential centrifugation and Bradford assay. Data represent means; error bars represent standard error; n = 6; *p = 0.0014, **p = 0.0052 by paired t-test.

https://doi.org/10.7554/eLife.04288.006
Figure 3—figure supplement 1
Effects of thermal stress and Hsp104 on protein accumulation.

(A) Lysates were isolated from [PSI+]Weak strains (SLL2600) incubated at 30°C, 37°C, 40°C, or 37°C before 40°C for 30 min and analyzed by SDS-PAGE and quantitative immunoblotting for Sup35. Data represent means; error bars represent standard deviations; n = 4. (B) Lysates were isolated from [PSI+]Weak strains (SLL2600) incubated at 30°C, 37°C, 40°C, or 37°C before 40°C for 30 min and analyzed by SDS-PAGE and quantitative immunoblotting for Hsp104, Ssa1, Sis1 or phosphoglycerate kinase (PGK) as a loading control (representative blot; see Figure 3A for quantification). (C) Lysates were isolated from a [PSI+]Weak strain containing a galactose-inducible HSP104 at the endogenous locus (SY1749) after galactose treatment and Hsp104 protein was quantified by SDS-PAGE and immunoblotting. Data represent means; error bars represent standard deviations; n = 3. (D) Galactose-inducible HSP104 [PSI+]Weak strains (SY1749) were grown in the presence of galactose for various times and plated on YPD for analysis of [PSI+] phenotype. Data represent means; error bars represent standard deviation; n = 3. (E) Lysates isolated from galactose-inducible HSP104 [PSI+]Strong (SY1748) or [PSI+]Weak (SY1749) cultures treated as described in (D) were analyzed by SDD-AGE and immunoblotting for Sup35. (F) Lysates were isolated from [PSI+]Strong (black) (SLL2606) and [psi] (white) (SLL2119) strains that were treated as described in (B), and heat-induced protein aggregates were quantified following differential centrifugation and Bradford assay. Data represent means; error bars represent standard errors; n ≥ 5. (G) Lysates were isolated from a [PSI+]Weak strain (SLL2600) that was incubated at 30°C or 40°C for 30 min in the absence (untreated) or presence of GdnHCl, and heat-induced protein aggregates were quantified following differential centrifugation and Bradford assay. Data represent means; error bars represent standard error; n = 3.

https://doi.org/10.7554/eLife.04288.007
Figure 4 with 1 supplement
Hsp104 engages heat-induced substrates upon thermal stress.

(A) A [PSI+]Weak strain with a GFP-tagged endogenous Hsp104 (SY2126) was incubated at 30°C, 37°C, 40°C, or 40°C with GdnHCl for 30 min, and immunocapture in the presence (+) or absence (−) of anti-GFP antibodies (Ab) was performed on native lysates. Proteins were analyzed by SDS-PAGE and general protein staining (Flamingo, top), or immunoblotting for GFP (bottom). (B) [PSI+]Weak (SY2126) or [psi] (SY2125) HSP104GFP strains were incubated at 30°C, 37°C, 40°C, or 37°C before 40°C for 90 min, and the pattern of Hsp104-GFP fluorescence was examined by microscopy. Scale bar = 1 μm. (C) Quantification of Hsp104-GFP fluorescence pattern in [PSI+]Weak (SY2126) cells, treated as described in (B): no localization (white); single dot (light gray); faint aggregate (medium gray); bright aggregate (dark gray); multiple bright aggregates (black); n > 25.

https://doi.org/10.7554/eLife.04288.008
Figure 4—figure supplement 1
Characterization of HSP104GFP strain.

(A) [PSI+]Weak (SLL2600) and [PSI+]Weak HSP104GFP (SY2126) strains were grown at 30°C, plated on YPD, and incubated at 30°C for analysis of [PSI+] colony color phenotype. (B) [PSI+]Weak (SLL2600, gray) and [PSI+]Weak HSP104GFP (SY2126, white) strains were incubated at 40°C for the indicated times and plated on YPD at 30°C for analysis of prion curing by colony color phenotype. Data represent means; error bars represent standard deviations; n = 3.(C) Lysates were isolated from WT (SLL2600) or HSP104GFP (SY2126) [PSI+]Weak strains that were incubated at 30°C or 40°C for 30 min, and heat-induced protein aggregates were quantified by differential centrifugation and Bradford assay. Data represent means; error bars represent standard error; n = 3. (D) Quantitative western blotting for Hsp104 was performed on lysates from [PSI+]Weak (SLL2600) and [PSI+]Weak HSP104GFP (SY2126) strains after incubation at 40°C for the indicated times. Data represent means; error bars represent standard deviations; n = 3. (E) Hsp104GFP and an mCherry-tagged firefly-luciferase (FFLmCh) reporter were visualized in a [PSI+]Weak strain (SY2802) by microscopy following incubation at 30°C or after a 30-min recovery from an incubation at 40°C for 90 min (30°C→40°C). Scale bar = 1 μm. (F) Hsp104GFP was visualized in a [PSI+]Weak strain (SY2126) by microscopy after a 90-min recovery from incubation at 40°C for 90 min in the absence (40°C) or presence of GdnHCl added before (GdnHCl→40°C) or after (40°C→GdnHCl) heat treatment. Scale bar = 1 μm. (G) [PSI+]Weak HSP104GFP cultures (SY2126) treated as described in (F) were plated on YPD and incubated at 30°C for analysis of [PSI+] colony color phenotype. Data represent means; error bars represent standard deviations; n = 3; *p = 0.0001,**p = 0.0089.

https://doi.org/10.7554/eLife.04288.009
Figure 5 with 1 supplement
Curing results from the asymmetric localization of Hsp104 following thermal stress.

(A) A [PSI+]Weak HSP104GFP culture (SY2126) was imaged over time in a microfluidics chamber at 30°C after a 30 min incubation at 30°C, 37°C, 40°C, or 37°C before 40°C. Fluorescence intensity in daughter and mother cells was quantified at the first cell division in cells that were budded (gray) or unbudded (orange) after thermal stress. Lines represent medians; boxes represent upper and lower quartiles, and whiskers represent maximum and minimum. All pairwise comparisons are significantly distinct, with a p < 0.015, except where indicated (N.S.), by unpaired t-test; n ≥ 10. (B) A [PSI+]Weak HSP104GFP WT (SY2126, gray) or BNI1 deletion strain (Δbni1) (SY2486, green) was imaged over time in a microfluidics chamber at 30°C after a 30 min incubation at 40°C. Fluorescence intensity in daughter and mother cells was quantified at the first cell division. Lines represent medians; boxes represent upper and lower quartiles; and whiskers represent maximum and minimum; n ≥ 14; p = 0.0075 by unpaired t-test. (C) [PSI+]Weak WT (SLL2600) or Δbni1 strains (SY1888), treated as described in (B), were plated on YPD to analyze curing by colony color phenotype. Data represent means; error bars represent standard deviations; n = 3; p < 0.0001 by unpaired t-test. (D) A [PSI+]Weak HSP104GFP strain (SY2126) was imaged over time in a microfluidics chamber at 30°C after a 30 min incubation at 40°C and with GdnHCl added before or after the 40°C incubation. Fluorescence intensity in daughter and mother cells was quantified at the first cell division. Lines represent medians; boxes represent upper and lower quartiles; and whiskers represent maximum and minimum; n > 11; *p = 0.0003, **p = 0.0026 by unpaired t-test. (E) A [PSI+]Weak strain (SLL2600) was incubated at 40°C for 30 min and plated on rich medium. Mother and daughter pairs were separated by micromanipulation and allowed to form colonies, which were then dispersed to YPD for analysis of curing by colony color phenotype. n = 15. (F) A [PSI+]Weak HSP104GFP culture (SY2126) was incubated at 30°C (dotted) or at 40°C for 30 min and allowed to recover for 30 min at 30°C (solid) before analysis of GFP fluorescence intensity by flow cytometry. Based on these intensities, cells were sorted into four fractions (orange, blue, purple, red) by FACS. (G) Cells collected in (F) were plated on YPD to analyze curing by colony color phenotype. Data represent means; error bars represent standard deviations; n = 2; *p = 0.02 by paired t-test.

https://doi.org/10.7554/eLife.04288.010
Figure 5—figure supplement 1
Characterization of chaperone asymmetric retention following thermal stress.

(A) A [psi] strain expressing heat-inducible untagged GFP (SY2091) was imaged over time in a microfluidics chamber at 30°C after 30 min incubation at 40°C (red) or 30°C (gray). Fluorescence intensity in daughter and mother cells was quantified at the first cell division in budded cells. Lines represent medians, boxes represent upper and lower quartiles, and whiskers represent maximum and minimum; n ≥ 11. (B) A [PSI+]Weak strain expressing a GFP-tagged endogenous Ssa1 and DsRedNLS (SY2659) was imaged after a 90 min incubation at 30°C, 37°C, 40°C, or 37°C before 40°C. Scale bar = 2 μm. (C) A [PSI+]Weak strain expressing a GFP-tagged endogenous Sis1 and DsRedNLS (SY2485) was imaged after a 90-min incubation at 30°C, 37°C, 40°C, or 37°C before 40°C. Scale bar = 2 μm. (D) A [PSI+]Weak SSA1GFP culture (SY2658) was imaged over time in a microfluidics chamber at 30°C after a 30 min incubation at 40°C (red) or 30°C (gray). Fluorescence intensity in daughter and mother cells was quantified at the first cell division in budded cells. Lines represent medians, boxes represent upper and lower quartiles, and whiskers represent maximum and minimum; n > 15. (E) A [PSI+]Weak SIS1GFP culture (SY2447) was imaged over time in a microfluidics chamber at 30°C after a 30 min incubation at 40°C (red) or 30°C (gray). Fluorescence intensity in daughter and mother cells was quantified at the first cell division in budded cells. Lines represent medians, boxes represent upper and lower quartiles, and whiskers represent maximum and minimum; n ≥ 7. (F) Quantitative immunoblotting for Hsp104 was performed on lysates from WT (SLL2600) or Δbni1 (SY1888) [PSI+]Weak cultures treated at 30°C (black) and 40°C (white) for 30 min following SDS-PAGE. Data represent means; error bars represent standard deviations; n = 3. (G) Lysates were isolated from WT (SLL2600) or Δbni1 (SY1888) [PSI+]Weak strains that were incubated at 30°C or 40°C for 30 min, and heat-induced protein aggregates were analyzed by differential centrifugation and Bradford assay. Data represent means; error bars represent standard error; n = 3.

https://doi.org/10.7554/eLife.04288.011
Figure 6 with 1 supplement
Efficient curing occurs in late cell-cycle staged cells following thermal stress.

(A) Single cells from an asynchronous WT [PSI+]Weak culture (SLL2600) were scored for morphology following bright-field imaging by microscopy: unbudded (black), tiny bud (dark gray), small bud (gray), medium bud (light gray), large bud (white). n = 153. (B) α-factor-arrested cultures were analyzed as in (A) over time after release. n ≥ 250. (C) Nocodazole-arrested cultures were analyzed as in (A) over time after release. n ≥ 175. (D) A [PSI+]Weak HSP104GFP strain (SY2126) released from α-factor arrest was incubated at 40°C (solid black lines) for 30 min before analysis by flow cytometry. 100,000 cells were analyzed per sample. (E) A [PSI+]Weak HSP104GFP strain (SY2126) released from nocodazole arrest was incubated at at 40°C (black lines) for 30 min before analysis by flow cytometry. 100,000 cells were analyzed per sample. (F) α-factor-arrested cultures (SLL2600) were incubated at 40°C for 30 min immediately or 30 min after release, and curing was quantified by colony color phenotype after plating on YPD at 30°C. Data represent means; error bars represent standard deviations; n = 3; p = 0.0255 by unpaired t-test. (G) Nocodazole-arrested cultures (SLL2600) were incubated at 40°C for 30 min immediately or 30 min after release, and curing was quantified colony color phenotype after plating on YPD at 30°C. Data represent means; error bars represent standard deviations; n = 3; p = 0.0263 by unpaired t-test.

https://doi.org/10.7554/eLife.04288.013
Figure 6—figure supplement 1
Characterization of chaperone accumulation and engagement in arrested cultures.

(A) Lysates were isolated from asynchronous, α-factor-arrested, or nocodazole-arrested [PSI+]Weak cultures (SLL2600) following incubation at 30°C (black) or 40°C (white) for 30 min, and the levels of Hsp104 were determined by quantitative immunoblotting following SDS-PAGE. Data represent means; error bars represent standard deviations; n = 3. (B) Asynchronous, α-factor-arrested, and nocodazole-arrested [PSI+]Weak HSP104GFP (SY2126) cultures were treated for 90 min at 30°C or 40°C and imaged by microscopy. Scale bar = 2 μm.

https://doi.org/10.7554/eLife.04288.014
Substrate–chaperone engagement must exceed time to cell division to induce curing.

(A) The number of [PSI+]Weak HSP104GFP (SY2126) cells containing fluorescent foci was quantified in cultures recovering at 30°C over time following a 90 min incubation at 40°C (white). Colony forming units in these cultures were quantified by plating (black). Data represent means; error bars represent standard deviations; n = 3. (B) [PSI+]Weak HSP104GFP cells (SY2126) treated for 30 min at 40°C and imaged over time in a microfluidics chamber are shown. Cells that were budded at the time of thermal stress are outlined in white, while unbudded cells are outlined in orange. Solid lines mark mothers, and dotted lines mark daughters. Scale bar = 1 µm. (C) A [PSI+]Weak HSP104GFP strain (SY2126) was imaged over time in a microfluidics at 30°C after a 30 min incubation at 40°C chamber. Budded or unbudded cells were scored at the first cell division for the presence or absence of fluorescent aggregates. Data represent means; error bars represent standard deviations; n = 3; p = 0.0005 by unpaired t-test.

https://doi.org/10.7554/eLife.04288.015
Model for Sup35 amyloid resolubilization and curing upon thermal stress.

Upon thermal stress, cellular proteins (green) misfold and aggregate, leading to the induction and recruitment of Hsp104 (barrel). If thermal stress occurs in unbudded cells (1), these aggregates are resolved prior to cell division, allowing the partitioning of Hsp104 to both mother (black) and daughter (gray) cells (left). If thermal stress occurs in budded cells (2), heat-induced aggregates persist upon cell division (3), leading to the asymmetric retention of Hsp104 in mother cells. Both heat-induced aggregates (green) and Sup35 amyloid (blue corkscrews) are resolved in cells accumulating high levels of Hsp104, leading to curing (red, 4).

https://doi.org/10.7554/eLife.04288.016

Tables

Table 1

Relative fluorescence intensity in mother cells

https://doi.org/10.7554/eLife.04288.012
Treatment (°C)Hsp104 (Relative to 30°C)Ssa1 (Relative to 30°C)Sis1 (Relative to 30°C)
30°→30°1 ± 0.1 (24)1 ± 0.2 (29)1 ± 0.1 (18)
30°→37°1.6 ± 0.2 (11)
30°→40°3.5 ± 0.6 (52)2.7 ± 0.5 (18)1.5 ± 0.1 (7)
37°→40°3.4 ± 0.4 (46)
  1. [PSI+]Weak HSP104GFP(SY2126), SSA1GFP (SY2658), or SIS1GFP (SY2447) cultures were treated at indicated temperatures and were imaged over time at 30°C using microfluidics and fluorescence microscopy. Average fluorescence intensity in mother cells with indicated standard deviations (±), which originated from budded cells at the time of thermal stress, was measured at the first cell division. Number of cells analyzed is indicated in parentheses. p values are <0.001 for all comparisons to 30°C treatment.

Table 2

Plasmids

https://doi.org/10.7554/eLife.04288.017
NameDescription
SB20pRS306-PSup35N(GS)3sGFP(GS)3MC
SB503pRS304-PGPDGST-DsRED-NLS
SB630pRS306-PGALHsp104
SB657pRS306-PtetO2Sup35
SB658pRS306-PtetO2Sup35(G58D)
SB849pRS306-PHSEGFP
SB1013pRS306-PGPDFFL-mCherry
Table 3

Primers

https://doi.org/10.7554/eLife.04288.018
NameSequence
5XbaI firefly5′-TCTAGAATGGAAGATGCCAAAAACATTAAG-3′
3BamHI firefly5′-GGATCCACCTTGAGACTGTGGTTGGAAAC-3′
5BamHI GS3mCherry5′-GGATCCGGTAGTGGTAGTGGTAGTATGGTGAGCAAGGG CGAGGAG-3′
3XhoI mCherry5′-CTCGAGTTACTTGTACAGCTCGTCCATGCCG-3′
SD275′-ACTTGCTCGGAATAACATCTATATCTGCCCACTAGCAACA CAGCTGAAGCTTCGTACGC-3′
SD285′-GGTATTATTGTGTTTGCATTTACTTATGTTTGCAAGAAATG CATAGGCCACTAGTGGATCTG-3′
Psup3525′-GAGATGCTCATCAAGGG-3′
PTEFCH5′-GCACGTCAAGACTGTCAAGG-3′
Sup35 3′chk5′-TATTTACGAAGGAGACCCGGAG-3′
pFa6 test5′-TGCCCAGATGCGAAGTTAAGTG-3′
HSP104-GFP F-A5′-CGATAATGAGGACAGTATGGAAATTGATGATGACCTA GATCGGATCCCCGGGTTAATTAA-3′
Hsp104-GFP R-A5′-TATTATATTACTGATTCTTGTTCGAAAGTTTTTAAAAATC GAATTCGAGCTCGTTTAAAC-3′
Hsp104for5′-GGCACATCCTGATGTTTTGA-3′
GFP-R5′-CCTTCACCCTCTCCACTGACAG-3′
Hsp104 3 flank R5′-CCGTATTCTAATAATGGACCAATC-3′
GFP-GS-Ssa1-F5′-AGCTCCAGAGGCTGAAGGTCCAACCGTTGAAGAAGTTG ATGGTTCTGGTTCTGGTTCTCGGATCCCCGGGTTAATTAA-3′
GFP-Ssa1-R5′-ACCCAGATCATTAAAAGACATTTTCGTTATTATCAATTGC GAATTCGAGCTCGTTTAAAC-3′
Sis1-GFP-F GS5′-ACTAAACGACGCTCAAAAACGTGCTATAGATGAAAATTT TGGTTCTGGTTCTGGTTCTCGGATCCCCGGGTTAATTAA-3′
Sis1-GFP-R5′-ATTTATTTGAGTTTATAATTATATTTGCTTAGGATTACTAG AATTCGAGCTCGTTTAAAC-3′
AD-BNI1-f5′-ATGTTGAAGAATTCAGGCTCCAAACATTCGAACTCAAAG GCAGCTGAAGCTTCGTACGC-3′
AD-BNI1-r5′-TTATTTGAAACTTAGCCTGTTACCTGTCCTAGCCTCACCT GCATAGGCCACTAGTGGATCTG-3′
AD-BNI1-fseq5′-GACATCGGTTAGAGGAAG-3′
AD-BNI1-rseq5′-CACTGTGCTTGTCACTTA-3′
Table 4

Yeast strains

https://doi.org/10.7554/eLife.04288.019
StrainGenotypePlasmids integratedReferenceFigure
SLL2119MATa [psi] ade1-14 his3Δ200 trp1-289 ura3-52 leu2-3, 112-Chernoff et al., 19951c, 3Sf
SLL2600MATa [PSI+]Weak ade1-14 his3Δ200 trp1-289 ura3-52 leu2-3, 112-Derkatch et al., 19961, 2a, 3, 5ce, 6abcfg, 1S, 3Sabg, 4Sabcd, 5Sfg, 6Sa
SLL2606MATa [PSI+]Strong ade1-14 his3Δ200 trp1-289 ura3-52 leu2-3, 112-Chernoff et al., 19951ac, 3Sf
SLL3071MATa/α [PSI+]Strong ade1-14/ade1-14 his3Δ200/his3Δ200 trp1-289/ trp1-289 ura3-52/ura3-52 leu2-3112/ leu2-3112-DiSalvo et al., 20112d
SLL3252MATa [psi] ade1-14 his3Δ200 trp1-289 ura3-52 leu2-3, 112-Chernoff et al., 1995‘Materials and methods’
SY86MATα [psi] ade1-14 his3Δ200 trp1-289 ura3-52 leu2-3, 112 sup35::N(GS)3GFP(GS)3MCSB20Derdowski et al., 2010‘Materials and methods’
SY197MATa [psi] ade1-14 his3-11,-15 trp1-1 ura3-1 leu2-3112 can1-100-J Weissman (YJW513)‘Materials and methods’
SY591MATa/α [PSI+]Weak ade1-14/ade1-14 his3Δ200/his3Δ200 TRP/ trp1-289 ura3-52/ura3-52 leu2-3112/ leu2-3112 HSP104/hsp104::LEU2-This study2b
SY782MATa/α [PSI+]Weak ade1-14/ade1-14 his3Δ200/his3Δ200 trp1-289/ trp1-289 ura3-52/ura3-52 leu2-3112/ leu2-3112 SUP35/sup35::N(GS)3GFP(GS)3MC-This study‘Materials and methods’
SY945MATa/α [PSI+]Weak ade1-14/ade1-14 his3Δ200/his3Δ200 trp1-289/ trp1-289 ura3-52/ura3-52 leu2-3112/ leu2-3112-This study2b
SY957MATa/α [PSI+]Strong ade1-14/ade1-14 his3Δ200/his3Δ200 trp1-289/ trp1-289 ura3-52/ura3-52 leu2-3112/ leu2-3112 SUP35/sup35::KANMX4-This study2d
SY1646MATa/α [PSI+]Strong ade1-14/ade1-14 his3Δ200/his3Δ200 trp1-289/ trp1-289 ura3-52/ura3-52::URA3::PtetO2SUP35 leu2-3112/ leu2-3112 SUP35/sup35::KANMX4SB657DiSalvo et al., 20112c
SY1648MATa/α [PSI+]Strong ade1-14/ade1-14 his3Δ200/his3Δ200 trp1-289/ trp1-289 ura3-52/ura3-52::URA3::PtetO2SUP35(G58D) leu2-3112/ leu2-3112 SUP35/sup35::KANMX4SB658DiSalvo et al., 20112c
SY1698MATα [PSI+]Strong ade1-14 his3Δ200 ura3-52 leu2-3 kar1-d15 ConR CyhR-This study‘Materials and methods’
SY1699MATα [PSI+]Weak ade1-14 his3Δ200 ura3-52 leu2-3 kar1-d15 ConR CyhR-This study‘Materials and methods’
SY1748MATa [PSI+]Strong ade1-14 his3-11,-15 trp1-1 ura3-1::URA3::PGALHSP104 leu2-3112 can1-100SB630This study3Se
SY1749MATa [PSI+]Weak ade1-14 his3-11,-15 trp1-1 ura3-1::URA3::PGALHSP104 leu2-3112 can1-100SB630This study3Scde
SY1888MATa [PSI+]Weak ade1-14 his3Δ200 trp1-289 ura3-52 leu2-3, 112 Δbni1::KANMX4-This study5c, 5Sfg
SY2091MATa [psi] ade1-14 his3Δ200 trp1-289 ura3-52::URA::PHSEGFP leu2-3, 112SB849This study5Sa
SY2125MATα [psi] ade1-14 his3Δ200 trp1-289 ura3-52 leu2-3112 HSP104GFP::KANMX6-This study4b
SY2126MATa [PSI+]Weak ade1-14 his3Δ200 trp1-289 ura3-52 leu2-3112 HSP104GFP::KANMX6-This study4, 5abdfg, 6de, 7, 4Sabcdfg, 6Sb
SY2447MATa [PSI+]Weak ade1-14 his3Δ200 trp1-289 ura3-52 leu2-3112 SIS1GFP::KANMX6-This study5Se
SY2485MATa [PSI+]Weak ade1-14 his3Δ200 trp1-289::TRP::PGPDGST-DsRed-NLS ura3-52 leu2-3112 SIS1GFP::KANMX6SB503This study5Sc
SY2486MATa [PSI+]Weak ade1-14 his3Δ200 trp1-289 ura3-52 leu2-3, 112 HSP104GFP::KANMX6 Δbni1::hphMX4-This study5b
SY2658MATa [PSI+]Weak ade1-14 his3Δ200 trp1-289 ura3-52 leu2-3112 SSA1GFP::KANMX6-This study5Sd
SY2659MATa [PSI+]Weak ade1-14 his3Δ200 trp1-289::TRP::PGPDGST-DsRed-NLS ura3-52 leu2-3112 SSA1GFP::KANMX6SB503This study5Sb
SY2802MATa [PSI+]Weak ade1-14 his3Δ200 trp1-289 ura3-52::URA::PGPDFirefly-mCherry leu2-3112 HSP104GFP::KANMX6SB1013This study4Se

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  1. Courtney L Klaips
  2. Megan L Hochstrasser
  3. Christine R Langlois
  4. Tricia R Serio
(2014)
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