doi: 10.1073/pnas.1102762108.
Epub 2011 Mar 14.
Suicidal [PSI+] is a lethal yeast prion
Affiliations
- PMID: 21402947
- PMCID: PMC3069153
- DOI: 10.1073/pnas.1102762108
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Suicidal [PSI+] is a lethal yeast prion
Proc Natl Acad Sci U S A.
.
Abstract
[PSI(+)] is a prion of the essential translation termination factor Sup35p. Although mammalian prion infections are uniformly fatal, commonly studied [PSI(+)] variants do not impair growth, leading to suggestions that [PSI(+)] may protect against stress conditions. We report here that over half of [PSI(+)] variants are sick or lethal. These "killer [PSI(+)]s" are compatible with cell growth only when also expressing minimal Sup35C, lacking the N-terminal prion domain. The severe detriment of killer [PSI(+)] results in rapid selection of nonkiller [PSI(+)] variants or loss of the prion. We also report variants of [URE3], a prion of the nitrogen regulation protein Ure2p, that grow much slower than ure2Δ cells. Our findings give a more realistic picture of the impact of the prion change than does focus on "mild" prion variants.
Conflict of interest statement
The authors declare no conflict of interest.
Figures
Screening of Ade+ colonies for killer [PSI+]. Isolated Ade+ colonies were restreaked three times on −Ade −Ura + 10 μg/mL doxycycline before being stamped on FOA. Circled colonies have killer [PSI+]. The fractions of isolates with mild, sick, and killer [PSI+] are shown below.
Killer [PSI+] strains are sick because of Sup35p deficiency. Cells carrying killer [PSI+], a nontoxic [PSI+], and a [psi−] control were streaked on ½YPD with (A) or without (B) doxycycline (10 μg/mL).
Toxicity and instability of [PSI+] isolates. (A) Sick and killer [PSI+] candidates were streaked on ½YPD and on FOA plates. After 2 d of growth on ½YPD, strains were restreaked on FOA plates. (B–D) Individual sick [PSI+] and nontoxic [PSI+] colonies were streaked on ½YPD from FOA. (Lower) Single colonies restreaked on ½YPD are indicated.
Multiple Sup35NM-GFP foci for killer [PSI+] and single foci for benign [PSI+]. (A) Newly induced 74-D694 [PSI+] colonies that could not grow on FOA plates (killer [PSI+]) were transformed with the pSupNM-GFP plasmid directly from −Ade −Ura + doxycycline plates. Transformants were selected only for the presence of pSupNM-GFP and were highly heterogeneous by color. White and sectoring transformants appeared as a result of the loss of the Sup35C plasmid, and their [PSI+] has become benign. Red transformants still carry the Sup35C-expressing plasmid and contained [PSI+] (probably killer [PSI+]), as was shown by fluorescent microscopy analysis. (B and C) Red transformants from A of two independent killer [PSI+] variants contain [PSI+] and show cells with multiple Sup35NM-GFP foci. (D) Typical white transformants from A and benign 74-D694 [PSI+] isolates show cells with mostly single Sup35NM-GFP foci. Six benign [PSI+] and four killer [PSI+] isolates were transformed as described in A. Transformants of both [PSI+] types that tend to retain the Sup35C plasmid were compared, and about 2,000 individual cells containing [PSI+] were analyzed for the presence of multiple Sup35NM-GFP foci per cell by fluorescent microscopy analysis. About 50% of putative killer [PSI+] cells had multiple foci, compared with only about 10% of benign [PSI+] cells under these conditions.
Spontaneously formed [URE3] clones with dramatically slowed growth and mitotic instability. BY241 (A), BY241 Δure2::TRP1 (B), BY241 individual spontaneously formed [URE3] colonies (C–F), and second streaks of small BY241 [URE3] colonies (G and H) from E and F. All strains were grown on ½YPD for 3 d before the pictures were taken.
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