Project description:To analyze phosphorylation sites of ALLO-1, worm eggs expressing GFP-ALLO-1 in the atg-11 or ikke-1 background were lysed in co-IP buffer, and GFP-ALLO-1 was immunoprecipitated with GFP-Trap-agarose beads. Proteins on the beads were directly digested with Trypsin overnight. Supernatants were collected, acidified to pH2.5 and desalted using GL-Tip SDB followed by LC-MS/MS analysis.

Project description:To analyze phosphorylation sites of ALLO-1, worm eggs expressing GFP-ALLO-1 in the atg-11 or ikke-1 background were lysed in co-IP buffer, and GFP-ALLO-1 was immunoprecipitated with GFP-Trap-agarose beads. Proteins on the beads were directly digested with Trypsin overnight. Supernatants were collected, acidified to pH2.5 and desalted using GL-Tip SDB followed by PRM analysis.

Project description:Wild-type or S2265A version of GFP-RIF1 protein (isoform 1) was over-expressed in Flp-In-T-REx cells (Watts et al. 2020. eLife 9:e58020) and immunopurified using GFP-Trap magnetic agarose beads. Proteins were subjected to on-beads trypsin digestion and resulting peptides were analysed by mass spectrometry for protein identification/quantification and identification of phosphorylated residues. Raw MS file names and descriptions: IP_RIF1_A.raw = GFP-RIF1-L immunoprecipitated from cells without aphidicolin treatment. IP_RIF1_B.raw = GFP-RIF1-L immunoprecipitated from cells treated with 1 µM aphidicolin for 24 hr before harvesting. IP_RIF1_C.raw = GFP-RIF1-L (S2265A) immunoprecipitated from cells treated with 1 µM aphidicolin for 24 hr before harvesting.

Project description:OfMasc-GFP derivatives or GFP were transiently expressed in OfTC cells. At 2 days post transfection, OfTC cells were treated with 100 nM Bortezomib for 1 day. The OfT1C cells were then fixed with 0.1% formaldehyde, and the fixation was quenched with 300 mM glycine. The cells were lysed on ice in 1 mL of RIPA buffer. After centrifugation, the supernatants were incubated with GFP-Trap Magnetic Agarose (ChromoTek) for 3 h at 4ºC. Proteins bound to the beads were digested by adding 200 ng of Trypsin/Lys-C mix (Promega) for 16 h at 37ºC. The digests were reduced, alkylated, acidified with trifluoroacetic acid, and desalted using a GL-Tip SDB (GL Sciences). LC-MS/MS analysis of the resultant peptides was performed using an EASY-nLC 1200 UHPLC connected to an Orbitrap Fusion mass spectrometer equipped with a nanoelectrospray ion source (Thermo Fisher Scientific). Raw data were directly analyzed against the wFur encoded protein data predicted from an in-house assembled wFur draft genomic sequence and O. furnacalis protein data ‘GCF_004193835.1_ASM419383v1_protein.faa’ downloaded from NCBI supplemented with OfMasc-GFP and GFP-Trap sequences using Proteome Discoverer version 2.4 (Thermo Fisher Scientific) with Sequest HT search engine. Label-free precursor ion quantification was performed using the precursor ions quantifier node.

Project description:Fertilized eggs (wild type or ikke-1 mutant) were collected from approximately 10,000 or 70,000 adult hermaphrodites, equivalent to 5 or 35 plates of 10-cm dish culture, at 60–72 h after the L1 stage using the bleaching method, and immediately frozen in liquid nitrogen. The eggs were thawed on ice in HEPES-RIPA3 buffer (20 mM HEPES-KOH pH 7.4, 150 mM NaCl, 1% [v/v] NP40, 0.25% [w/v] Na-deoxycholate, 0.05% [w/v] SDS, and 50 mM NaF) with Complete EDTA-free Protease Inhibitor Cocktail (Roche, Basel, Switzerland) and PhosSTOP (Roche). The eggs were sonicated, incubated for 15 min at 4°C, and centrifuged at 16,200 ×g for 15 min at 4°C. The supernatant was collected and centrifuged at 16,200 ×g for 10 min at 4°C. The supernatant was transferred to a fresh tube, and GFP-Trap magnetic agarose beads (Proteintech, Rosemont, IL, USA) that had been prewashed with HEPES-RIPA3 buffer were added. The beads and supernatant were rotated for 2 h at 4°C. After rotation, the beads were transferred to a Protein LoBind tube (Eppendorf, Hamburg, Germany), washed three times with HEPES-RIPA3 buffer, and washed twice with 50 mM ammonium bicarbonate. The beads were divided to three new Protein LoBind tube with 50 µL of 50 mM ammonium bicarbonate. The proteins on the beads were digested using three methods. A) Beads and 200 ng of trypsin/LysC mix (Promega) were mixed and shaken overnight at 37°C. B) Beads and 200 ng of chymotrypsin (Roche) were mixed and shaken with 10 mM CaCl2 overnight at 25°C. C) Beads and 40 ng of Asp-N (Promega) were mixed and shaken overnight at 37°C. After the reaction, supernatants containing the digested peptides were collected, reduced, alkylated, acidified to pH 2.5 with TFA, and desalted using GL-Tip SDB (GL Sciences, Tokyo, Japan). The eluates were evaporated and dissolved in 3% ACN and 0.1% TFA. LC-MS/MS analysis of the resulting peptides was performed on an EASY-nLC 1200 UHPLC system connected to an Orbitrap Fusion mass spectrometer using a nanoelectrospray ion source (Thermo Fisher Scientific). The peptides were separated on a C18 reversed-phase column with a linear 4–32% ACN gradient for 0–100 min, followed by an increase to 80% ACN for 10 min, which was held at 80% ACN for 10 min. The mass spectrometer was operated in data-dependent acquisition mode with a maximum duty cycle of 3 s. The MS1 spectra were measured at a resolution of 60,000, an AGC target of 4e5, and a mass range of 350–1500 m/z. HCD MS/MS spectra were acquired using an Orbitrap with a resolution of 30,000, AGC target of 5e4, isolation window of 1.6 m/z, maximum injection time of 54 ms, and normalized collision energy of 30. Dynamic exclusion was set to 15 s. Raw data were directly analyzed against the C. elegans WormBase protein database supplemented with the EPG-7-GFP sequence using Proteome Discoverer 2.4 (Thermo Fisher Scientific) with the Sequest HT search engine. The search parameters were as follows: (a) trypsin, chymotrypsin, or Asp-N as an enzyme with up to two, three, or three missed cleavages, respectively; (b) precursor mass tolerance of 10 ppm; (c) fragment mass tolerance of 0.02 Da; (d) carbamidomethylation of cysteine as a fixed modification; (e) acetylation of the protein N-terminus, oxidation of methionine, and phosphorylation of serine, threonine, and tyrosine as variable modifications. Peptides were filtered at a false discovery rate of 1% using Percolator node. Label-free quantification was performed based on the intensities of the precursor ions using a precursor-ion quantifier node.

Project description:To identify the potential interaction partners of PRSS37, three testis lysates of Prss37E/+ mice (PRSS37-EGFP knock-in heterozygous mice) and three testis lysates of pAcr-EGFP transgenic mice were immunoprecipitated using anti-GFP mAb magnetic beads. The GFP-IP products of six samples from two groups were subsequently analyzed by mass spectrometry (MS) to identify differentially immmunoprecipitated proteins (DIPs) in the PRSS37-EGFP group. Proteins detected in pAcr-EGFP group were used as negative controls to exclude the endogenous proteins and polypeptides that interact nonspecifically with the anti-GFP mAb magnetic beads.

Project description:YFP-NPH3 was immunoprecipitated with GFP-Trap-A agarose beads from transgenic Arabidopsis plants, and then phosphorylation sites of NPH3 were identified.

Project description:We immunoprecipitated exogengusly expressed TaRACK1B-GFP，TaSGT1-GFP and TaHSP90-GFP fused protein in wheat protoplasts.A high-throughput technology, LC-MS/MS, was applied to identify the candidate interacting proteins of TaRACK1B-GFP，TaSGT1-GFP and TaHSP90-GFP

Project description:RNAseq of GFP-sorted cells (Low-GFP vs. High-GFP, GFP-fed vs GFP+fed)

Project description:GFP or GFP-200 proteins were purified from the corresponding Flp-In™ T REx™ 293 cells using GFP-Trap beads. Purified proteins were analyzed by mass spectrometry.