Construction of the RapiDeg yeast strain

Protocol for “Construction of the RapiDeg yeast strain”

1. Plasmids

MLP479: pRS305-pTDH3-FRB-3xUb  (see attached vector map)

MLP379:pFA6a-GFP-2xFKBP-TRP1  (see attached vector map)

2. Strains

SEY6210: MATα, ura3-52 his3Δ-200 leu2-3,112 trp1-901 lys2-801suc2Δ9(Robinson et al., 1988)

SEY6210.1: MATa, ura3-52 his3Δ-200 leu2-3,112 trp1-901 lys2-801suc2Δ9(Robinson et al., 1988)

LZY273: SEY6210.1;tor1-1 fpr1Δ::natMX

LZY562:  SEY6210.1;tor1-1  fpr1Δ::natMX  leu2–3,112::pRS305-PTDH3FRB-3xUb CAN1::CAN1-GFP-2xFKBP-TRP VPH1::VPH1-mCherry-kanMX6

3. Growth media

YPD media: Yeast extract, 1% (mv); Peptone, 2% (m/v); agar (for plate use only, 2%(m/v)); dextrose, 2%(m/v).

Yeast synthetic growth media: Yeast nitrogen base (with (NH₄)₂SO₄), 0.67% (m/v); supplemented with necessary amino acids; agar (for plate use only, 2%(m/v)); dextrose, 2%(m/v).

4. Generating and validating the RapiDeg strain

When necessary, gene deletion and tagging were made using standard yeast genetic replacement technique with longtine-based PCR cassettes (Longtine et al., 1998).

4.1 Construct the RapiDeg parent strain

(1) WT strains (SEY6210 or SEY6210.1) were made rapamycin-resistant by transforming a PCR fragment encoding the dominant TOR1 mutant (S1972I) and selected for growth on YPD plates (supplemented with 1 μg/ml rapamycin). The tor1-1 mutant was further validated by rapamycin resistance and TOR1 sequence.

(2) FPR1 (FKBP-12) gene was knocked out to ensure pairing of FRB-3xUb to target proteins tagged with FKBP.

4.2 Cargo protein tagging

(1) Design the primers to C-terminally tag the protein of interest with GFP-2xFKBP, using MLF379 as the template;

(2) PCR amplify the C-terminal tagging fragment with homology to the C-terminus of the cargo protein. In the RapiDeg parent strain constructed in the step 4.1, perform standard genetic procedures to fuse the protein of interest with a C-terminal GFP-2xFKBP and culture the yeast on appropriate selection plate. 

4.3 Cargo sorting assay

(1) The strain generated in the 4.2 will be further transformed with FRB-3xUb expression vector MLP479 and empty vector pRS305 as a negative control;

(2) Culture this RapiDeg strain (Cargo protein is tagged with C-terminal GFP-2xFKBP) co-expressing the FRB-3xUb in either YPD or appropriate minimal medium. Grow the culture to mid-log phase (OD₆₀₀~0.6) and add rapamycin to 1μg/mL (final working concentration).  Collect the cells for fluorescence microscopy and western blot analysis.

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