What Do I Need for Successful Method Development?
Presentations | 2020 | Agilent TechnologiesInstrumentation
Effective method development in high-performance liquid chromatography is essential for delivering fast, sensitive and reproducible analyses in pharmaceutical, environmental, food and metabolomics laboratories. Careful selection of column chemistry, particle size, mobile phase composition and instrument configuration underlies routine quality control and advanced research workflows.
This application note outlines a systematic approach to reversed-phase method development, illustrating how to choose columns, particles and mobile phase modifiers, optimize gradients and instrument parameters to achieve required resolution and speed. Case studies using Agilent InfinityLab Poroshell 120 columns demonstrate efficiency gains and robustness across a range of analytes.
Key steps in the development plan include:
Comparative studies highlight that superficially porous particles reduce run times from 35 min to under 9 min while maintaining or improving resolution. Resolution is most sensitive to selectivity (α), underscoring the impact of bonded phase choice and mobile phase pH. Lower dwell volumes and minimized tubing ID increase peak sharpness and reproducibility. Implementing wash procedures and deactivator additives prevents analyte adsorption on steel surfaces, restoring signal for polar and phosphorylated metabolites.
The described workflow accelerates method development, reduces solvent consumption and improves method robustness. Laboratories benefit from:
Emerging trends include wider adoption of sub-2 µm superficially porous particles at moderate pressures, integration of digital diagnostic tools for automated optimization, and expanded use of PEEK-lined and deactivated flow paths for bioanalytical and metabolomics applications. Novel stationary phases and continuous-flow microfluidics promise further gains in throughput and selectivity.
A structured method development plan encompassing column chemistry, particle size, mobile phase optimization and instrument configuration delivers efficient, high-resolution separations suitable for diverse analytical challenges. Attention to extra-column effects, robust fittings and routine column benchmarking ensures reproducibility and simplifies method transfer.
HPLC
IndustriesManufacturerAgilent Technologies
Summary
Importance of the Topic
Effective method development in high-performance liquid chromatography is essential for delivering fast, sensitive and reproducible analyses in pharmaceutical, environmental, food and metabolomics laboratories. Careful selection of column chemistry, particle size, mobile phase composition and instrument configuration underlies routine quality control and advanced research workflows.
Objectives and Study Overview
This application note outlines a systematic approach to reversed-phase method development, illustrating how to choose columns, particles and mobile phase modifiers, optimize gradients and instrument parameters to achieve required resolution and speed. Case studies using Agilent InfinityLab Poroshell 120 columns demonstrate efficiency gains and robustness across a range of analytes.
Methodology and Instrumentation
Key steps in the development plan include:
- Column selection: start with C18 bonded phases on superficially porous particles (2.7 µm) for balanced performance below instrument pressure limits.
- Particle size: evaluate 4 µm for standard HPLC, 2.7 µm for UHPLC-like performance, and 1.9 µm for maximum efficiency when high pressure is available.
- Mobile phase: use simple aqueous–organic mixtures (formic or acetic acid in water, acetonitrile or methanol as modifier) with pH control to tune retention of ionizable compounds.
- Gradient conditions: apply an initial linear gradient (e.g. 5–95 % organic) then refine slope, hold and re-equilibration times to meet retention (k′ ≥ 1) and resolution (Rs ≥ 2) targets.
- Instrument setup: optimize dwell volume, extra-column dispersion, data acquisition rate, detector bandwidth and sampling rate to preserve sharp peaks and accurate efficiency measurements.
Used Instrumentation
- Agilent 1100 and 1260 Infinity II LC systems with diode array detectors.
- Agilent 1290 Infinity II pumps (binary and quaternary) for precise gradient control and reduced dwell volume.
- Agilent InfinityLab Poroshell 120 columns (C18, SB-C18, HPH-C18, CS-C18 and alternative chemistries) in various dimensions.
- Spring-loaded Quick Connect and Quick Turn fittings for low-dead-volume, tool-free column installation.
Main Results and Discussion
Comparative studies highlight that superficially porous particles reduce run times from 35 min to under 9 min while maintaining or improving resolution. Resolution is most sensitive to selectivity (α), underscoring the impact of bonded phase choice and mobile phase pH. Lower dwell volumes and minimized tubing ID increase peak sharpness and reproducibility. Implementing wash procedures and deactivator additives prevents analyte adsorption on steel surfaces, restoring signal for polar and phosphorylated metabolites.
Benefits and Practical Applications
The described workflow accelerates method development, reduces solvent consumption and improves method robustness. Laboratories benefit from:
- Faster turnaround with shorter columns and optimized gradients.
- Greater sensitivity for early-eluting peaks and ionizable compounds via pH tuning and inert hardware.
- Scalable methods through consistent column chemistries and reproducible manufacturing quality.
Future Trends and Possibilities for Use
Emerging trends include wider adoption of sub-2 µm superficially porous particles at moderate pressures, integration of digital diagnostic tools for automated optimization, and expanded use of PEEK-lined and deactivated flow paths for bioanalytical and metabolomics applications. Novel stationary phases and continuous-flow microfluidics promise further gains in throughput and selectivity.
Conclusion
A structured method development plan encompassing column chemistry, particle size, mobile phase optimization and instrument configuration delivers efficient, high-resolution separations suitable for diverse analytical challenges. Attention to extra-column effects, robust fittings and routine column benchmarking ensures reproducibility and simplifies method transfer.
Reference
- Agilent Application Note 5990-5572EN: Poroshell vs. Totally Porous Particles Comparison.
- Agilent Application Note 5994-2358EN: Alternative C18 Selectivity Evaluation.
- Agilent Application Note 5994-2274EN: Mobile Phase pH Effects on CS-C18.
- Agilent Application Note 5991-7560EN: Column Efficiency vs. Data Rate.
- Agilent Application Note 5988-6476EN: Effect of Mobile Phase Preparation on Chromatography.
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