Proteins were expressed in cell-free systems using E-PCR2 product

Proteins were expressed in cell-free systems using E-PCR2 products as template with E. coli lysates which were prepared as described before ( Broedel et al., 2013). A typical 50 μl standard reaction comprised 35% (v/v) E. coli lysate containing T7

RNA-polymerase, 40% learn more reaction buffer containing complete amino acids (1.2 mM each), 25× XE-solution (EasyXpress linear template Kit Plus, Qiagen), 9 μl linear E-PCR2 product and 14C-labeled leucine (Perkin Elmer, Leucine, L-[14C(U)], final concentration: 50 μM; 4 DPM/pmol). Coupled transcription-translation reactions were performed in a thermomixer (37 °C, 500 rpm) for 90 min, followed by a detailed analysis described in 2.5. To determine the toxin’s integrity and functionality an aliquot of a nonradioactive crude reaction mixture (CRM) and the supernatant (SN) was analyzed by hemolysis and RPLA agglutination

assays. Hemolytic activity of cell-free synthesized toxins was determined as described below. The total yield and soluble protein was determined by hot trichloroacetic acid (TCA)-precipitation. Total protein yield was determined from CRM and soluble protein in the supernatant (SN) which was obtained after a 10 min centrifugation step at 16,000× g at PS341 room temperature. After synthesis, 5 μl aliquots of the translation reactions (CRM and SN) were stopped by the addition of 3 ml TCA (10% solution with 2% casein hydrolysate). To precipitate newly synthesized proteins and to hydrolyze the amino acids on charged tRNAs, samples containing TCA were placed in boiling water for 15 min and then cooled in ice for 30 min. TCA-precipitated proteins were collected on filters (Machery-Nagel, MN GF-3). Protein loaded filters were washed twice with TCA (5% solution w/o casein hydrolysate) and rinsed twice with acetone. Dry filters were GBA3 placed in scintillation vials and subsequently 3 ml scintillation cocktail (Zinsser Analytic, Quicksafe A) was added. Radioactivity was measured and zero-time blank was subtracted from radioactive samples

(Beckmann Coulter, LS 6500 Multi Purpose Scintillation Counter). To determine the homogeneity and size of in vitro translated proteins, 5 μl aliquots of radioactively labeled cell-free synthesis reactions (CRM and SN) were diluted in water (1:10) 0.150 μl ice-cold acetone was added and probes were incubated on ice for 15 min. Samples were centrifuged at 16,000× g for 5 min at 4 °C. The protein pellet was resuspended in 20 μl sample buffer (Life technologies, LDS-sample buffer) and subjected under reducing conditions to 10% Bis-Tris NuPAGE Novex gel (Life technologies). Subsequently, the gel was dried for 1 h and exposed to storage phosphor screens (GE Healthcare, Mounted GP) for 24 h. Radioactively labeled proteins were visualized using a phosphor-imager (Typhoon Trio+, GE Healthcare). Purification of His-tagged TDH proteins was performed using the Dynabeads®-His-tag Isolation and Pulldown Kit according to the manufacturer’s recommendation (Invitrogen, Darmstadt, Germany).

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