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3 protocols using anti rabbit igg h l hrpo

1

Protein Expression and Detection Protocol

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GFP-tagged proteins were recognized with a monoclonal α-GFP antibody (Roche; 1:1000) and arginine methylation was recognized with a monoclonal α-mono and dimethyl arginine antibody (Ab412, Abcam; 1:500), followed by a secondary α-mouse-horseradish peroxidase (HRP) antibody (GE Lifesciences; 1:5000). Slr1-TAP was recognized with an HRP-conjugated goat anti-Protein A (PrA) antiserum (Rockland; 1:10,000). Ribosomal protein Rps3 was recognized with a polyclonal rabbit antibody against Rps3 (1:1000). Proteins were visualized through enhanced chemiluminescence (Pierce) and autoradiography.
Anti-rabbit IgG (H+L)-HRPO and anti-mouse IgG (H+L) HRPO (Dianova) secondary antibodies were used for sucrose density gradient fraction immunoblots. The signals were detected with Amersham ECL Prime Western Blotting Detection Reagent (GE Healthcare) and the FUSION-SL chemiluminescence detection system (Peqlab) and the Western blot analyses were quantified using the Image StudioLite software (LI-COR).
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2

Immunoblotting and Quantification of Methylated Proteins

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GFP‐tagged proteins were recognized with a monoclonal α‐GFP antibody (Roche; 1:1000) and arginine methylation was recognized with a monoclonal α‐mono and dimethyl arginine antibody (Ab412, Abcam; 1:500), followed by a secondary α‐mouse‐horseradish peroxidase (HRP) antibody (GE Lifesciences; 1:5000). Slr1‐TAP was recognized with an HRP‐conjugated goat anti‐Protein A (PrA) antiserum (Rockland; 1:10,000). Ribosomal protein Rps3 was recognized with a polyclonal rabbit antibody against Rps3 (1:1000). Proteins were visualized through enhanced chemiluminescence (Pierce) and autoradiography.
Anti‐rabbit IgG (H + L)‐HRPO and anti‐mouse IgG (H + L) HRPO (Dianova) secondary antibodies were used for sucrose density gradient fraction immunoblots. The signals were detected with Amersham ECL Prime Western Blotting Detection Reagent (GE Healthcare) and the FUSION‐SL chemiluminescence detection system (Peqlab) and the Western blot analyses were quantified using the Image StudioLite software (LI‐COR).
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3

Characterization of Yeast Ribosomal Proteins

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Polyclonal rabbit antibodies against Rpl35 (kindly provided by M. Seedorf, dilution 1:5000), Hem15 and Aco1 (kindly provided by R. Lill, dilution 1:7000 and 1:2000 respectively), Mex67 (kindly provided by C. Dargemont, dilution 1:50000), Rio2 (kindly provided by K. Karbstein, dilution 1:2000), Dbp5 (dilution 1:1000) and Rps3 (dilution 1:1000) were used. GFP-tagged proteins were detected with an anti-GFP antibody (sc-8334; Santa Cruz, dilution 1:1000) and myc-tagged proteins with an anti-myc antibody (sc-789; Santa Cruz, dilution 1:750). Monoclonal mouse antibodies against Pab1 (Santa Cruz, dilution 1:1000) and GST (sc-138; Santa Cruz, dilution 1:2000) and secondary anti-rabbit IgG (H+L)-HRPO and anti-mouse IgG (H+L)-HRPO (Dianova) antibodies were used. The signals were detected with Amersham ECL Prime Western Blotting Detection Reagent (GE Healthcare) and the FUSION-SL chemiluminescence detection system (Peqlab) and the Western blot analyses were quantified using the Bio1D software (Peqlab).
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