Surfactant Cocktail-Aided Extraction/Precipitation/On-Pellet Digestion Strategy Enables Efficient and Reproducible Sample Preparation for Large-Scale Quantitative Proteomics

Shen, Shichen; An, Bo; Wang, Xue; Hilchey, Shannon P.; Li, Jun; Cao, Jun; Tian, Yu; Hu, Chenqi; Jin, Lina; Ng, Andrew; Tu, Chengjian; Qu, Miao; Zand, Martin S.; Qu, Jun

doi:10.1021/acs.analchem.8b02172

“…Multiple variations on protein extraction and digestion were tested, based on the highest percent recovery of peptides per milligram of starting plant material by use of an absorbance (562 nm) assay for tryptic peptides (Pierce BCA Protein Assay Kit Cat# 23225) (data not shown). The final sample method was based on the filter-aided sample preparation method (FASP, Expedeon SKU:44250) [37]. Briefly, 1 mg of fresh plant flower was flash frozen at −80 • C for 20 min.…”

Section: Sample Preparationmentioning

confidence: 99%

The Cannabis Proteome Draft Map Project

Jenkins

¹

,

Orsburn

²

2020

IJMS

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Recently we have seen a relaxation of the historic restrictions on the use and subsequent research on the Cannabis plants, generally classified as Cannabis sativa and Cannabis indica. What research has been performed to date has centered on chemical analysis of plant flower products, namely cannabinoids and various terpenes that directly contribute to phenotypic characteristics of the female flowers. In addition, we have seen many groups recently completing genetic profiles of various plants of commercial value. To date, no comprehensive attempt has been made to profile the proteomes of these plants. We report herein our progress on constructing a comprehensive draft map of the Cannabis proteome. To date we have identified over 17,000 potential protein sequences. Unfortunately, no annotated genome of Cannabis plants currently exists. We present a method by which “next generation” DNA sequencing output and shotgun proteomics data can be combined to produce annotated FASTA files, bypassing the need for annotated genetic information altogether in traditional proteomics workflows. The resulting material represents the first comprehensive annotated protein FASTA for any Cannabis plant. Using this annotated database as reference we can refine our protein identifications, resulting in the confident identification of 13,000 proteins with putative function. Furthermore, we demonstrate that post-translational modifications play an important role in the proteomes of Cannabis flower, particularly lysine acetylation and protein glycosylation. To facilitate the evolution of analytical investigations into these plant materials, we have created a portal to host resources developed from our proteomic and metabolomic analysis of Cannabis plant material as well as our results integrating these resources.

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“…SEPOD utilizes a high‐concentration surfactant cocktail (SC) buffer containing multiple non‐ionic/anionic surfactants (e.g., SDS, SDC, IGEPAL CA‐630), which are then removed by precipitation with organic solvent (e.g., acetone). The detergent cocktail achieves three important goals: (i) exhaustive/reproducible protein extraction, including MPs from cells and tissues; for example, the SC buffer significantly outcompeted SDT buffer in protein extraction from lung and brain, suggesting the use of multiple surfactants may afford more efficient disruption of cellular compartments and thereby enhancing protein extraction from tissues (Shen et al, ); (ii) effective removal of detrimental non‐protein matrix components (e.g., fatty acids, phospholipids, etc.) which would otherwise compromise the robustness of digestion and LC‐MS analysis; (iii) highly effective proteolytic digestion owing to the through, dual‐action (surfactants + precipitation) denaturation.…”

Section: Important Considerations For Ms1‐based Quantification In Larmentioning

confidence: 99%

“…which would otherwise compromise the robustness of digestion and LC‐MS analysis; (iii) highly effective proteolytic digestion owing to the through, dual‐action (surfactants + precipitation) denaturation. Compared with FASP and in‐solution digestion, SEPOD showed substantially higher peptide/protein (including MPs) recovery and ∼20–40% more peptide identifications, as well as improved quantification of peptides with extreme physicochemical properties in large sample cohorts (Shen et al, ). More importantly, the procedure enabled highly efficient, reproducible and robust preparation of large sample cohorts, as exemplified by analysis of 44 lung tissue samples in a time‐course investigation post virus infection (Shen et al, ).…”

Section: Important Considerations For Ms1‐based Quantification In Larmentioning

confidence: 99%

MS1 ion current‐based quantitative proteomics: A promising solution for reliable analysis of large biological cohorts

Wang¹,

Shen²,

Rasam

³

et al. 2019

Mass Spectrometry Reviews

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The rapidly‐advancing field of pharmaceutical and clinical research calls for systematic, molecular‐level characterization of complex biological systems. To this end, quantitative proteomics represents a powerful tool but an optimal solution for reliable large‐cohort proteomics analysis, as frequently involved in pharmaceutical/clinical investigations, is urgently needed. Large‐cohort analysis remains challenging owing to the deteriorating quantitative quality and snowballing missing data and false‐positive discovery of altered proteins when sample size increases. MS1 ion current‐based methods, which have become an important class of label‐free quantification techniques during the past decade, show considerable potential to achieve reproducible protein measurements in large cohorts with high quantitative accuracy/precision. Nonetheless, in order to fully unleash this potential, several critical prerequisites should be met. Here we provide an overview of the rationale of MS1‐based strategies and then important considerations for experimental and data processing techniques, with the emphasis on (i) efficient and reproducible sample preparation and LC separation; (ii) sensitive, selective and high‐resolution MS detection; iii)accurate chromatographic alignment; (iv) sensitive and selective generation of quantitative features; and (v) optimal post‐feature‐generation data quality control. Prominent technical developments in these aspects are discussed. Finally, we reviewed applications of MS1‐based strategy in disease mechanism studies, biomarker discovery, and pharmaceutical investigations.

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“…The final sample method was based on the filter-aided sample preparation method (FASP). 14 Briefly, 1mg of fresh plant material was flash frozen at -80°C for 20 minutes. The cell walls were disrupted by immediately removing the frozen material and blunt physical concussion.…”

Section: Sample Preparationmentioning

confidence: 99%

The Cannabis Multi-Omics Draft Map Project

Jenkins

¹

,

Orsburn

²

2019

Preprint

View full text Add to dashboard Cite

Recently we have seen a relaxation of the historic restrictions on the use and subsequent research on the Cannabis plants, generally classified as Cannabis sativa and Cannabis indica. What research has been performed to date has centered on chemical analysis of plant flower products, namely cannabinoids and various terpenes that directly contribute to phenotypic characteristics of the female flowers. In addition, we have seen many groups recently completing genetic profiles of various plants of commercial value. To date, no comprehensive attempt has been made to profile the proteomes of these plants. We report herein our progress on constructing a comprehensive draft map of the Cannabis proteome. To date we have identified over 17,000 potential protein sequences. Unfortunately, no annotated genome of Cannabis plants currently exists. We present a method by which "next generation" DNA sequencing output and shotgun proteomics data can be combined to produce annotated FASTA files, bypassing the need for annotated genetic information altogether in traditional proteomics workflows. The resulting material represents the first comprehensive annotated FASTA for any Cannabis plant. Using this annotated database as reference we can refine our protein identifications, resulting in the confident identification of 13,000 proteins with putative function. Furthermore, we demonstrate that posttranslational modifications play an important role in the proteomes of Cannabis flower, particularly lysine acetylation and protein glycosylation. To facilitate the evolution of analytical investigations into these plant materials, we have created a portal to host resources we have developed from proteomic and metabolomic analysis of Cannabis plant material as well as our results integrating these resources. All data for this project is available to view or download at www.CannabisDraftMap.Org Proteomics is a science dedicated to the creation of comprehensive quantitative snapshots of all the proteins produced by an individual organism, tissue or cell. 1 The term was coined in the 1990s during the efforts to sequence the first complete human genomes. 2 While the technology was in place to complete the human genome draft in 2003, the first two drafts of the human proteome were not completed by teams led by Johns Hopkins and CIPSM researchers until 2014. These two separate and ambitious projects were the composite of thousands of hours of instrument run time utilizing the most sophisticated hardware available at that time. 3,4 Recent advances in mass spectrometry technology now permit the completion of proteome profiles in more practical time. Single celled organisms have been "fully" sequenced in less than an hour, and by use of multi-dimensional chromatography, relatively high coverage human proteomes have been completed in only a few days. 5-7 While much can be learned by sequencing DNA and RNA in a cell, quantifying and sequencing the proteome has distinct advantages as proteins perform physical and enzymatic activities in the cell and ar...

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Surfactant Cocktail-Aided Extraction/Precipitation/On-Pellet Digestion Strategy Enables Efficient and Reproducible Sample Preparation for Large-Scale Quantitative Proteomics

Cited by 38 publications

References 47 publications

The Cannabis Proteome Draft Map Project

The Cannabis Proteome Draft Map Project

MS1 ion current‐based quantitative proteomics: A promising solution for reliable analysis of large biological cohorts

The Cannabis Multi-Omics Draft Map Project

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