Chromatographic Separation Theory
Chromatographic separation theory explains how analytes migrate and bands broaden, providing the figures of merit that quantify a separation's quality.
Definition
Chromatographic separation theory is the body of physical-chemical principles that describes analyte retention and band broadening in chromatography and quantifies separation performance through retention, selectivity, efficiency, and resolution.
Scope
This topic covers the conceptual framework common to all chromatographic methods: the retention factor and distribution constant, selectivity, the plate model of efficiency, the rate theory's account of band broadening, and the resolution equation that ties these together. It is the theoretical complement to the technique-specific topics of gas, liquid, and electrophoretic separation.
Core questions
- How are retention factor, selectivity, and plate count defined and measured?
- What physical processes broaden chromatographic bands as analytes migrate?
- How does the rate theory predict an optimum mobile-phase velocity?
- How does the resolution equation combine efficiency, selectivity, and retention?
Key theories
- Plate theory
- Modeling the column as a series of equilibrium stages gives the number of theoretical plates and the plate height as measures of efficiency; sharper, more numerous plates correspond to narrower peaks, and the concept derives from Martin and Synge's partition treatment.
- Rate (van Deemter) theory
- The rate theory expresses plate height as a sum of eddy diffusion, longitudinal diffusion, and mass-transfer resistance terms that vary with flow velocity, predicting a minimum plate height at an optimal velocity and explaining how particle size and diffusion limit efficiency.
Mechanisms
An analyte's distribution constant between mobile and stationary phases sets its retention factor and thus its elution time. Selectivity is the ratio of retention factors for two analytes and reflects differences in chemistry. As bands migrate they spread through eddy diffusion in the packing, longitudinal molecular diffusion, and finite rates of mass transfer between phases; the rate theory sums these into plate height. The resolution of two peaks then follows from the interplay of efficiency, selectivity, and retention.
Clinical relevance
Separation theory guides practical method development everywhere chromatography is used—choosing column dimensions, particle size, and flow rate to achieve the resolution and speed needed for pharmaceutical, environmental, clinical, and food analyses.
History
The theoretical foundation began with Martin and Synge's 1941 partition-chromatography paper, which introduced the plate concept and earned them the Nobel Prize. Van Deemter and colleagues' 1956 rate theory connected plate height to physical transport processes, and Giddings later unified and extended the kinetic theory of band broadening.
Key figures
- Archer Martin
- Richard Synge
- Jan van Deemter
- John Calvin Giddings
Related topics
Seminal works
- martin1941
- vandeemter1956
- skoog2017
Frequently asked questions
- What is a theoretical plate?
- It is a conceptual unit of separation efficiency borrowed from distillation; a column with more theoretical plates produces narrower peaks, and plate count is calculated from a peak's retention time and width.
- Why is there an optimal flow rate in chromatography?
- The rate theory shows that band broadening from longitudinal diffusion decreases with faster flow while mass-transfer broadening increases, so plate height is lowest—and efficiency highest—at an intermediate, optimal velocity.