UW Nunn Lab - Coho Salmon Ovary DIA

UW Nunn Lab - Coho Salmon Ovary DIA
DIA Proteomics of Coho Salmon Ovaries Across 4 Stages
Data License: CC BY 4.0 | ProteomeXchange: PXD052361 | doi: https://doi.org/10.6069/2aak-qf86
  • Organism: Oncorhynchus kisutch
  • Instrument: Orbitrap Fusion Lumos
  • SpikeIn: No
  • Keywords: coho, salmon, gametogenesis, reproduction
  • Lab head: Brook L. Nunn Submitter: Emma Timmins-Schiffman
Abstract
A better understanding of coho salmon ovarian maturation will inform both aquaculture and conservation efforts. Ovarian maturation is a complex molecular and physiological process resulting in a mature ovum that can be released for spawning and fertilization. The confluence of molecular signals and pathways that must be co-expressed to accomplish full reproductive maturity with high quality oocytes have been previously investigated with with low-resolution proteomics and transcriptomics. This dataset expands proteomics resources for coho salmon by thousands of proteins, allowing for a more in-depth assessment of the range of proteins involved in ovarian maturation and their interactions. We sampled coho salmon at four ovarian developmental stages that encompass the transition from primary to secondary (vitellogenic) growth. Data independent acquisition proteomics was applied to the dataset, resulting in the inference of >5000 proteins in the coho ovarian proteome.
Experiment Description
Female coho salmon were reared in a hatchery and sacrificed for ovarian dissection at time points corresponding to the following ovarian stages: early perinucleolar (EPN), late perinucleolar (LPN), early cortical alveolus (ECA), and late cortical alveolus (LCA). Tissues were stored at -80C until processing. Ovarian tissues were homogenized in an ammonium bicarbonate + SDS lysis buffer using a bullet blender. Proteins were extracted and digested using S-trap mini columns from Protifi. Liquid chromatography was run in-line with the mass spectrometer to separate peptides before MS/MS analysis. The fused silica pre-column, with an in-house made kasil frit, was 3.5 cm long with a 150 µm i.d. and the in-house pulled fused silica analytical column was 34 cm long with a 75 µm i.d. Both columns were packed with Dr. Masich C18 3 µm beads in-house. The Lumos mass spectrometer (Thermo Fisher) was run in data independent acquisition (DIA) mode. The pooled samples were analyzed with narrow window (2 m/z) DIA in gas-phase fractions (400-500 m/z, 500-600, 600-700, 700-800, 800-900, 900-1000) to generate an in-depth spectral library. Individual ovary peptide samples were analyzed with wider window DIA (8 m/z) across the m/z range of X-Y. Sample order was randomized for mass spectrometry analysis and between each 3-4 samples a QC (PRTC + BSA) and a solvent blank were run. Mass spectrometry results were analyzed using the Prosit-EncyclopeDIA-Skyline pipeline described in Searle et al. (2020). Raw mass spectrometry files were converted to .mzML format in MSConvert with the following parameters: remove titleMaker filter, write index, TPP compatibility, use zlib compression, SIM as spectra, and added filters with default settings (peakPicking and demultiplex). The database used for peptide detection was the predicted coho proteome (GCF_002021735.2_Okis_V2.protein.faa). We discovered the some proteins of interest for ovarian maturation were not included in this proteome, so we added sequences for follicle stimulating hormone (FSH), luteinizing hormone (LH), the receptors for FSH and LH, two 5-alpha reductases, and an ovarian aromatase. All sequences were derived from coho salmon, except for the FSH receptor, which came from the Atlantic salmon proteome. The coho proteome was converted to a prosit csv in EnclycopeDIA v. 1.4.10 and the .csv was subdivided into five sub-proteomes since Prosit has a file size limit. Prosit creates theoretical spectral libraries that frequently improve peptide detections in our pipeline. Each prosit .txt file was downloaded and converted to .dlib format in EncyclopeDIA v.1.4.10. The five .dlibs were combined into a single file for further analyses.
Sample Description
coho salmon ovaries
Created on 5/17/24, 10:32 PM
Clustergrammer Heatmap
 
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06_Refinement-Method_Pooled-Sample_2024-12-12_13-01-05.sky.zip2025-04-01 14:47:211467671,0164
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04_Present-in-positive_Single-Runs_2024-12-11_10-53-50.sky.zip2025-04-01 14:47:09141022054,5446
03_Confirmation__Pooled-Sample_2024-12-11_10-46-23.sky.zip2025-04-01 14:47:06141092194,8341
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050924withassaymapcurves_2025-04-01_15-31-03.sky.zip2025-04-01 12:31:261484862
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calibration_CRP_ESDTSYVSLK.sky.zip2025-03-10 14:38:04112645
calibration_IgG3_TPLGDTTHTCPR.sky.zip2025-03-10 14:38:04112633
calibration_SAA4_EALQGVGDMGR.sky.zip2025-03-10 14:38:04112630
calibration_SAA4_FRPDGLPK.sky.zip2025-03-10 14:38:04112633
calibration_A1AG2_SDVMYTDWK.sky.zip2025-03-10 14:38:04112633
calibration_ApoA_DYVSQFEGSALGK+AKPALEDLR.sky.zip2025-03-10 14:38:041241039
calibration_A1AT-1_AVLTIDEK.sky.zip2025-03-10 14:38:04112636
calibration_IgA1_TPLTATLSK.sky.zip2025-03-10 14:38:04112636
calibration_ApoE_LGPLVEQGR.sky.zip2025-03-10 14:38:04112642
calibration_CRP-1_GYSIFSYATK.sky.zip2025-03-10 14:38:04112430
calibration_SAA2-1_LTGHGAEDSLADQAANK+GPGGAWAAEVISNAR.sky.zip2025-03-10 14:38:041241242
calibration_SAA2-1_GAEDSLADQAANK.sky.zip2025-03-10 14:38:04112648
calibration_SAA1+2_SFFSFLGEAFDGAR.sky.zip2025-03-10 14:38:04112639
calibration_SAA1+2_EANYIGSDK.sky.zip2025-03-10 14:38:04112642
calibration_A1AG1_NWGLSVYADKPETTK.sky.zip2025-03-10 14:38:04112633
calibration_CX3CL1_AQDGGPVGTELFR.sky.zip2025-03-10 14:38:04112645
calibration_CHGA_VAHQLQALR.sky.zip2025-03-10 14:38:04112639
calibration_SERPINF2_FDPSLTQR+DFLQSLK.sky.zip2025-03-10 14:38:041241248
calibration_SERPINF2-1_LGNQEPGGQTALK.sky.zip2025-03-10 14:38:04112639
calibration_B2M_VNHVTLSQPK.sky.zip2025-03-10 14:38:04112639
calibration_CAL2_DLQNFLK.sky.zip2025-03-10 14:38:04112645
calibration_SAA1_FFGHGAEDSLADQAANEWGR.sky.zip2025-03-10 14:38:04112633
calibration_A1AG2_TLMFGSYLDDEK.sky.zip2025-03-10 14:38:04112639
calibration_IgG2_GLPAPIEK.sky.zip2025-03-10 14:38:04112648
calibration_IgG_total_NQVSLTCLVK+DTLMISR.sky.zip2025-03-10 14:38:041241257
calibration_IgG1_TTPPVLDSDGSFFLYSK+GPSVFPLAPSSK.sky.zip2025-03-10 14:38:041241257
calibration_A1AT-1_FNKPFVFLMIEQNTK.sky.zip2025-03-10 14:38:04112636
calibration_IgG3_SCDTPPPCPR.sky.zip2025-03-10 14:38:04112642
calibration_MPO_QNQIAVDEIR+VVLEGGIPILR.sky.zip2025-03-10 14:38:041241242
calibration_MPO_IANVFTNAFR.sky.zip2025-03-10 14:38:04112639
calibration_CAL2_LGHPDTLNQGEFK.sky.zip2025-03-10 14:38:04112642
calibration_CAL1_ALNSIIDVYHK+GADVWFK.sky.zip2025-03-10 14:38:041241239
calibration_IgG4_TTPPVLDSDGSFFLYSR+GLPSSIEK.sky.zip2025-03-10 14:38:041241239
calibration_KNG1_QVVAGLNFR.sky.zip2025-03-10 14:38:041121042
calibration_KNG1_TVGSDTFYSFK+YFIDFVAR.sky.zip2025-03-10 14:38:041242048
calibration_AMBP_GVCEETSGAYEK+ETLLQDFR.sky.zip2025-03-10 14:38:041242048
calibration_LBP_ITLPDFTGDLR+LAEGFPLPLLK.sky.zip2025-03-10 14:38:041241848
calibration_CST3_ALDFAVGEYNK.sky.zip2025-03-10 14:38:04112848
calibration_A2M_AIGYLNTGYQR.sky.zip2025-03-10 14:38:04112645
calibration_A2M_NEDSLVFVQTDK.sky.zip2025-03-10 14:38:04112639
calibration_HP_TEGDGVYTLNNEK+VGYVSGWGR.sky.zip2025-03-10 14:38:031241245
calibration_CHGA_ELQDLALQGAK.sky.zip2025-03-10 14:38:03112648
calibration_SAA4_GPGGVWAAK.sky.zip2025-03-10 14:38:03112648
calibration_A1AG1_YVGGQEHFAHLLILR+TYMLAFDVNDEK.sky.zip2025-03-10 14:38:031241251
calibration_A1AG2_EHVAHLLFLR.sky.zip2025-03-10 14:38:03112442
calibration_A1AG1+2_WFYIASAFR.sky.zip2025-03-10 14:38:03112645
calibration_A1AT_SVLGQLGITK.sky.zip2025-03-10 14:38:03112639
calibration_A1AT_LSITGTYDLK+FLENEDR.sky.zip2025-03-10 14:38:031241251
Intra- and interday precision_part 2.sky.zip2025-03-07 14:34:0212234613818
Intra- and interday precision_part 1.sky.zip2025-03-07 14:34:0214285616818
Long-term QC_digested plasma.sky.zip2025-03-07 14:34:0214234613629
calibration_SAA1_FFGHGAEDSLADQAANEWGR.sky.zip2025-03-07 14:34:02112636
calibration_A1AG2_TLMFGSYLDDEK.sky.zip2025-03-07 14:34:02112636
calibration_IgG_total_NQVSLTCLVK+DTLMISR.sky.zip2025-03-07 14:34:021241260
calibration_IgG2_GLPAPIEK.sky.zip2025-03-07 14:34:02112651
calibration_IgG1_TTPPVLDSDGSFFLYSK+GPSVFPLAPSSK.sky.zip2025-03-07 14:34:021241260
calibration_A1AT-1_FNKPFVFLMIEQNTK.sky.zip2025-03-07 14:34:02112639
calibration_CAL2_LGHPDTLNQGEFK.sky.zip2025-03-07 14:34:02112551
calibration_MPO_VVLEGGIDPILR.sky.zip2025-03-07 14:34:02112648
calibration_MPO_QNQIAVDEIR.sky.zip2025-03-07 14:34:02112651
calibration_MPO_IANVFTNAFR.sky.zip2025-03-07 14:34:02112645
calibration_CAL1_ALNSIIDVYHK+GADVWFK.sky.zip2025-03-07 14:34:021241251
calibration_ApoE_LGPLVEQGR.sky.zip2025-03-07 14:34:02112651
calibration_SAA2-1_GPGGAWAAEVISNAR.sky.zip2025-03-07 14:34:02112639
calibration_SAA2-1_GAEDSLADQAANK+LTGHGAEDSLADQAANK.sky.zip2025-03-07 14:34:021241251
calibration_SAA1+2_EANYIGSDK.sky.zip2025-03-07 14:34:02112648
calibration_CRP_ESDTSYVSLK.sky.zip2025-03-07 14:34:02112651
calibration_IgG3_SCDTPPPCPR.sky.zip2025-03-07 14:34:02112651
calibration_IgG4_GLPSSIEK.sky.zip2025-03-07 14:34:02112651
calibration_IgG4_TTPPVLDSDGSFFLYSR.sky.zip2025-03-07 14:34:02112648

A better understanding of coho salmon ovarian maturation will inform both aquaculture and conservation efforts. Ovarian maturation is a complex molecular and physiological process resulting in a mature ovum that can be released for spawning and fertilization. The confluence of molecular signals and pathways that must be co-expressed to accomplish full reproductive maturity with high quality oocytes have been previously investigated with with low-resolution proteomics and transcriptomics. This dataset expands proteomics resources for coho salmon by thousands of proteins, allowing for a more in-depth assessment of the range of proteins involved in ovarian maturation and their interactions. We sampled coho salmon at four ovarian developmental stages that encompass the transition from primary to secondary (vitellogenic) growth. Data independent acquisition proteomics was applied to the dataset, resulting in the inference of >5000 proteins in the coho ovarian proteome. 

Female coho salmon were reared in a hatchery and sacrificed for ovarian dissection at time points corresponding to the following ovarian stages: early perinucleolar (EPN), late perinucleolar (LPN), early cortical alveolus (ECA), and late cortical alveolus (LCA). Tissues were stored at -80C until processing. Ovarian tissues were homogenized in an ammonium bicarbonate + SDS lysis buffer using a bullet blender. Proteins were extracted and digested using S-trap mini columns from Protifi. Liquid chromatography was run in-line with the mass spectrometer to separate peptides before MS/MS analysis. The fused silica pre-column, with an in-house made kasil frit, was 3.5 cm long with a 150 µm i.d. and the in-house pulled fused silica analytical column was 34 cm long with a 75 µm i.d. Both columns were packed with Dr. Masich C18 3 µm beads in-house. The Lumos mass spectrometer (Thermo Fisher) was run in data independent acquisition (DIA) mode. The pooled samples were analyzed with narrow window (2 m/z) DIA in gas-phase fractions (400-500 m/z, 500-600, 600-700, 700-800, 800-900, 900-1000) to generate an in-depth spectral library. Individual ovary peptide samples were analyzed with wider window DIA (8 m/z) across the m/z range of X-Y. Sample order was randomized for mass spectrometry analysis and between each 3-4 samples a QC (PRTC + BSA) and a solvent blank were run.

Mass spectrometry results were analyzed using the Prosit-EncyclopeDIA-Skyline pipeline described in Searle et al. (2020). Raw mass spectrometry files were converted to .mzML format in MSConvert with the following parameters: remove titleMaker filter, write index, TPP compatibility, use zlib compression, SIM as spectra, and added filters with default settings (peakPicking and demultiplex).


The database used for peptide detection was the predicted coho proteome (GCF_002021735.2_Okis_V2.protein.faa). We discovered the some proteins of interest for ovarian maturation were not included in this proteome, so we added sequences for follicle stimulating hormone (FSH), luteinizing hormone (LH), the receptors for FSH and LH, two 5-alpha reductases, and an ovarian aromatase. All sequences were derived from coho salmon, except for the FSH receptor, which came from the Atlantic salmon proteome. The coho proteome was converted to a prosit csv in EnclycopeDIA v. 1.4.10 and the .csv was subdivided into five sub-proteomes since Prosit has a file size limit. Prosit creates theoretical spectral libraries that frequently improve peptide detections in our pipeline. Each prosit .txt file was downloaded and converted to .dlib format in EncyclopeDIA v.1.4.10. The five .dlibs were combined into a single file for further analyses.


The combined .dlib is used as the library for chromatogram library construction in EnclycopeDIA v. 1.12.34. The background is the fasta file with all the protein sequences used to create the Prosit library. The pooled GPF samples (in mzML format) are used to generate an .elib chromatogram library file. This .elib is then used as the library to search the single injection, wide window .mzML files. The quant report resulting from these peptide detections becomes the library in the Skyline document. Search results and single injection .mzML files were imported into Skyline daily v. 22.2.1.256 (MacLean et al., 2010).



Female coho salmon ovaries