Microflow SWATH® Acquisition for Industrialized Quantitative Proteomics
Technical notes | 2017 | SCIEXInstrumentation
Data-independent acquisition (DIA) methods such as SWATH® have emerged as essential tools for large-scale quantitative proteomics, offering consistent peptide coverage and high reproducibility. As biomarker studies and industrial proteomic applications demand analysis of hundreds to thousands of samples, there is a critical need for workflows that balance sensitivity, robustness and throughput. Microflow liquid chromatography (LC) represents a promising compromise, delivering increased sample throughput with only a modest loss in sensitivity compared to traditional nanoflow LC.
This study evaluates the performance of microflow LC coupled with SWATH® acquisition on the NanoLC™ 400 and TripleTOF® 6600 systems. Key aims include assessing proteome coverage, quantitation precision and operational robustness relative to established nanoflow protocols, and identifying optimized conditions for industrialized proteomic workflows.
The experimental workflow comprised:
Key findings include:
The microflow SWATH® workflow delivers:
Advancements may include further integration with automated sample handling, expansion to clinical biomarker validation and adaptation to higher flow rates or multiplexed LC setups. Enhanced data analysis pipelines and real-time QC monitoring will support even larger cohort studies in drug development and precision medicine.
Microflow LC combined with SWATH® acquisition on the TripleTOF® 6600 system offers an efficient, reproducible and scalable proteomic platform. Under optimized conditions (8 μg load, 100 variable windows, high resolution mode), nearly 5 000 proteins can be quantified in a one-hour run, representing a robust solution for high-throughput industrial proteomics.
LC/TOF, LC/HRMS, LC/MS, LC/MS/MS
IndustriesProteomics
ManufacturerSCIEX
Summary
Significance of the Topic
Data-independent acquisition (DIA) methods such as SWATH® have emerged as essential tools for large-scale quantitative proteomics, offering consistent peptide coverage and high reproducibility. As biomarker studies and industrial proteomic applications demand analysis of hundreds to thousands of samples, there is a critical need for workflows that balance sensitivity, robustness and throughput. Microflow liquid chromatography (LC) represents a promising compromise, delivering increased sample throughput with only a modest loss in sensitivity compared to traditional nanoflow LC.
Objectives and Study Overview
This study evaluates the performance of microflow LC coupled with SWATH® acquisition on the NanoLC™ 400 and TripleTOF® 6600 systems. Key aims include assessing proteome coverage, quantitation precision and operational robustness relative to established nanoflow protocols, and identifying optimized conditions for industrialized proteomic workflows.
Methodology and Used Instrumentation
The experimental workflow comprised:
- Chromatography: A NanoLC™ 425 system operating at 5 μL/min on a 0.3 × 150 mm ChromXP™ column. A 43-minute gradient (4–32 % solvent B) enabled one-hour total runs with injected protein loads from 1 to 8 μg.
- Mass Spectrometry: SWATH® acquisition on a TripleTOF® 6600 with Turbo V™ source and 25 μm hybrid electrodes. Variable Q1 windows were defined using Analyst® TF 1.7, comparing high sensitivity (>15 000 resolution) and high resolution (>30 000 resolution) MS/MS modes.
- Data Processing: PeakView® SWATH® 2.0 with the Pan Human library. Quantitation was filtered at <1% false discovery rate (FDR) and <20% coefficient of variation (CV) across five replicates.
Main Results and Discussion
Key findings include:
- Retention Time Robustness: Analysis of 48 plasma samples over 2.5 days showed RT deviations of ≤10 s, enabling narrow SWATH® extraction windows.
- MS/MS Mode Optimization: High resolution mode increased quantified proteins by 5–15% versus high sensitivity mode on two instruments.
- Sample Load Effects: Increasing on-column load to 8 μg yielded 4 500–5 000 proteins quantified per hour, consistent across three systems.
- Window Strategy: Moving from 60 to 100 variable Q1 windows (with 75 to 40 ppm extraction widths and 25 ms accumulation) improved reproducible protein IDs by ~8% and peptides by ~17%, while maintaining CV performance.
- Microflow vs Nanoflow Comparison: Microflow SWATH® achieved ~85% of nanoflow protein coverage with fourfold higher throughput (24 vs 6 samples/day).
Benefits and Practical Applications
The microflow SWATH® workflow delivers:
- High Throughput: Up to 24 one-hour runs per day (~150 proteomes weekly).
- Robust Quantitation: >90% of peptides at <20% CV, dynamic range spanning four orders of magnitude.
- Operational Ease: Reduced system clogging, simpler connections and faster column re-equilibration compared to nanoflow.
Future Trends and Potential Applications
Advancements may include further integration with automated sample handling, expansion to clinical biomarker validation and adaptation to higher flow rates or multiplexed LC setups. Enhanced data analysis pipelines and real-time QC monitoring will support even larger cohort studies in drug development and precision medicine.
Conclusion
Microflow LC combined with SWATH® acquisition on the TripleTOF® 6600 system offers an efficient, reproducible and scalable proteomic platform. Under optimized conditions (8 μg load, 100 variable windows, high resolution mode), nearly 5 000 proteins can be quantified in a one-hour run, representing a robust solution for high-throughput industrial proteomics.
References
- Improved Data Quality Using Variable Q1 Window Widths in SWATH® Acquisition, SCIEX Technical Note RUO-MKT-02-2879-A
- Evolution of SWATH® Acquisition Provides Large Gains in Quantified Proteins, SCIEX Technical Note RUO-MKT-02-5772-A
- Exploring the Sensitivity Differences for Peptide Quantification in the Low Flow Rate Regime, SCIEX Technical Note RUO-MKT-02-3252-A
- Rosenberger G et al. Scientific Data (2014) 1, 140031
- Acknowledgment to Liu et al., ETH Zurich for HEK lysate preparation
- Accelerating SWATH® Acquisition for Protein Quantitation, SCIEX Technical Note RUO-MKT-02-8432-A
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