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The Essential CHROMacademy Guide Mobile Phase Optimization Strategies for Reversed Phase HPLC

Mobile Phase Optimization Strategies for Reversed Phase … · Chromatography in a future Essential Guide! When all else fails!! Question and Answer Type your question in the “Submit

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Page 1: Mobile Phase Optimization Strategies for Reversed Phase … · Chromatography in a future Essential Guide! When all else fails!! Question and Answer Type your question in the “Submit

The Essential CHROMacademy Guide

Mobile Phase Optimization Strategies forReversed Phase HPLC

Page 2: Mobile Phase Optimization Strategies for Reversed Phase … · Chromatography in a future Essential Guide! When all else fails!! Question and Answer Type your question in the “Submit

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Page 3: Mobile Phase Optimization Strategies for Reversed Phase … · Chromatography in a future Essential Guide! When all else fails!! Question and Answer Type your question in the “Submit

Speakers

Kevin SchugHPLC Dept. DeanCHROMacademy

Tony TaylorTechnical DirectorCHROMacademy

Moderator

Dave WalshEditor In ChiefLCGC Magazine

Page 4: Mobile Phase Optimization Strategies for Reversed Phase … · Chromatography in a future Essential Guide! When all else fails!! Question and Answer Type your question in the “Submit
Page 5: Mobile Phase Optimization Strategies for Reversed Phase … · Chromatography in a future Essential Guide! When all else fails!! Question and Answer Type your question in the “Submit

Mobile Phase Optimization Strategiesfor Reversed Phase HPLC

Page 6: Mobile Phase Optimization Strategies for Reversed Phase … · Chromatography in a future Essential Guide! When all else fails!! Question and Answer Type your question in the “Submit

1. Review of Reversed Phase Retention Mechanisms

2. Methanol or Acetonitrile - which one is best?

3. Eluotropic Strength - quick ways to reach the ideal!

4. Changing Solvent - useful tools and approaches

5. Mobile phase pH - understand the effects

6. Optimising pH vs. retention

7. Which buffer - what strength?

8. Strategies for when all else fails

Aims & Objectives

Page 7: Mobile Phase Optimization Strategies for Reversed Phase … · Chromatography in a future Essential Guide! When all else fails!! Question and Answer Type your question in the “Submit

1. Mobile Phase - mixture of organic and aqueous solvents

2. Stationary phase -hydrophobic moiety chemically bonded to silica

3. Mobile phase MORE POLAR than Stationary Phase

4. Analyte ‘partitions’ between the two phases depending upon its chemistry (hydrophobicity)

5. Increasing the % organic in the mobile phase increases the ‘elution power’ of the mobile phase

6. Retention and Selectivity are altered by changing the chemistry of the stationary phase mobile phase and the temperature

Reversed Phase Retention Mechanisms

Page 8: Mobile Phase Optimization Strategies for Reversed Phase … · Chromatography in a future Essential Guide! When all else fails!! Question and Answer Type your question in the “Submit

Controlling Retention and Selectivity

Retention and Selectivity are altered by changing:

Stationary Phase - chain length and chemistry, inclusion of polar moieties, exposure of silanol surface, polar end capping reagents

Mobile Phase - organic solvent type, % organic, pH, buffers and other additives

Temperature - especially with ionisable analytes

Page 9: Mobile Phase Optimization Strategies for Reversed Phase … · Chromatography in a future Essential Guide! When all else fails!! Question and Answer Type your question in the “Submit

Solvents for Reversed Phase HPLC (I)

1. Acetonitrile has lower viscosity - reduces back pressure and often results in slightly better peak shape

2. Acetonitrile has lower UV cut-off - advantage for UV detection

3. Methanol is less expensive and less toxic

4. Methanol is more polar - reducing the risks of solid buffer precipitation

Page 10: Mobile Phase Optimization Strategies for Reversed Phase … · Chromatography in a future Essential Guide! When all else fails!! Question and Answer Type your question in the “Submit

Solvents for Reversed Phase HPLC (II)

1. Acetonitrile forms binary mixtures with water

2. Methanol is ‘protic’ and can undergo polar polar / ionic interactions with solutes

3. Usually results in better selectivity for more polar compounds - at the expense of longer run times and increased peak asymmetry

4. Acetonitrile shows good wetting properties when low % B gradients are required - better early peak retention time reproducibility

MeOH MeCN

Page 11: Mobile Phase Optimization Strategies for Reversed Phase … · Chromatography in a future Essential Guide! When all else fails!! Question and Answer Type your question in the “Submit

Effect of Organic Modifier on Retention

Neutral HPLC Test Compound Mixtures - Selectivity also changes

Page 12: Mobile Phase Optimization Strategies for Reversed Phase … · Chromatography in a future Essential Guide! When all else fails!! Question and Answer Type your question in the “Submit

Selecting Optimum Eluotropic Strength (1)

1. Carry out separation at high %B (80%)

2. This saves time vs. starting at low pH

3. Reduce by 5-10% B in steps to assess retention

4. Look out for changes in selectivity

5. Really only works for neutral compounds

6. Ionisable species need to employ pH control

Page 13: Mobile Phase Optimization Strategies for Reversed Phase … · Chromatography in a future Essential Guide! When all else fails!! Question and Answer Type your question in the “Submit

MobilePhase_01.flv

Page 14: Mobile Phase Optimization Strategies for Reversed Phase … · Chromatography in a future Essential Guide! When all else fails!! Question and Answer Type your question in the “Submit

Scouting Gradient Methods

If Dtg < 0.25 tG then isocratic analysis is possible !

Isocratic composition:

tr(avg) = ti + tf /2

tr(avg) = 12.8 + 21.2 / 2

tr(avg) = 17.0 mins.

At 17.0 mins. eluent composition = 80% B

(Note: account for dwell volume!)

That’s the ‘BEST ESTIMATE’ isocratic composition for this separation

We will discuss the pH of the mobile phase and choice of buffer shortly

Page 15: Mobile Phase Optimization Strategies for Reversed Phase … · Chromatography in a future Essential Guide! When all else fails!! Question and Answer Type your question in the “Submit

Simulation to Optimise %B

1. Use modelling for predicting separation

2. This DryLab® model was achieved using 2 injections at 30% B and 50% B

Mixture of 6 Neutral Compounds

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MobilePhase_02.flv

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Altering Selectivity

1. What if separation isn’t achieved with the ‘OPTIMUM’ isocratic composition from the scouting gradient?

2. Adjust %B either side of optimum by 5-10% B

3. Use an alternative solvent to adjust selectivity

Page 18: Mobile Phase Optimization Strategies for Reversed Phase … · Chromatography in a future Essential Guide! When all else fails!! Question and Answer Type your question in the “Submit

Iso-Eluotropic Mobile Phases

1. Iso-eluotropic - same elution power

2. Iso-eluotropic solvents elute analytes in the same time frame with different selectivity

3. Can use an iso-eluogram(nomogram) to find iso-eluotropic solvent compositions

Page 19: Mobile Phase Optimization Strategies for Reversed Phase … · Chromatography in a future Essential Guide! When all else fails!! Question and Answer Type your question in the “Submit

MobilePhase_03.flv

Page 20: Mobile Phase Optimization Strategies for Reversed Phase … · Chromatography in a future Essential Guide! When all else fails!! Question and Answer Type your question in the “Submit

Mobile phase pH effects

1. pH reflects the hydrogen ion (or hydroxonium ion) concentration in solution

2. Adding acid (proton donor), increases the hydrogen ion concentration (lowers pH) of the solution

3. Adding base (proton acceptor), lowers the hydrogen ion concentration (increases pH) of the solution

Page 21: Mobile Phase Optimization Strategies for Reversed Phase … · Chromatography in a future Essential Guide! When all else fails!! Question and Answer Type your question in the “Submit

MobilePhase_04.flv

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Extent of Analyte Ionisation

1. Extent of analyte ionisation changes with mobile phase pH

2. Le Chateliers principle applies to the equilibrium when adding acidic or basic species to the mobile phase

3. Ionised form is more polar -less well retained under reversed phase conditions

4. Non-ionised (ion-suppressed form) is less polar - retained longer under reversed phase conditions

pKa = 50% Ionised (pH 4.6)

Page 23: Mobile Phase Optimization Strategies for Reversed Phase … · Chromatography in a future Essential Guide! When all else fails!! Question and Answer Type your question in the “Submit

MobilePhase_05.flv

Page 24: Mobile Phase Optimization Strategies for Reversed Phase … · Chromatography in a future Essential Guide! When all else fails!! Question and Answer Type your question in the “Submit

MobilePhase_06.flv

Page 25: Mobile Phase Optimization Strategies for Reversed Phase … · Chromatography in a future Essential Guide! When all else fails!! Question and Answer Type your question in the “Submit

Retention Control using Mobile Phase pH

Page 26: Mobile Phase Optimization Strategies for Reversed Phase … · Chromatography in a future Essential Guide! When all else fails!! Question and Answer Type your question in the “Submit

Optimising Separations using pH

What pH? Nicotine pKa? Robustness?

Page 27: Mobile Phase Optimization Strategies for Reversed Phase … · Chromatography in a future Essential Guide! When all else fails!! Question and Answer Type your question in the “Submit

Simulation to Optimise pH

1. Use modelling for predicting separation

2. This DryLab® model was achieved using 5 runs injections at: pH 2.9 / 3.0 / 3.5 / 5.0 / 6.5

Mixture of Acidic and Neutral Analytes

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MobilePhase_07.flv

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Buffers for Reversed Phase HPLC (I)

1. A ‘buffer’ - an aqueous solution of a mixture of a weak acid and its conjugate base or a weak base and its conjugate acid. pH of a buffered solution changes very little when a small amount of strong acid or base is added to it.

2. Where on the HPLC system do we expect pH to change?

3. Buffer capacity is critical -work within 1pH unit of the buffer pKa!! 20% of maximum buffer capacity is critical!

Page 30: Mobile Phase Optimization Strategies for Reversed Phase … · Chromatography in a future Essential Guide! When all else fails!! Question and Answer Type your question in the “Submit

Buffers for Reversed Phase HPLC (II)

4. 25-50mM is a good starting point for buffer solution concentration

5. Chose appropriate conjugate acid or base!

6. Always buffer the aqueous component of the mobile phase separately

7. pH of the mobile phase and pKa of analyte will change in the presence of organic solvents -consistency is the key!

Page 31: Mobile Phase Optimization Strategies for Reversed Phase … · Chromatography in a future Essential Guide! When all else fails!! Question and Answer Type your question in the “Submit

Buffers for Reversed Phase HPLC (III)

8. Increase buffer concentration or capacity if peak shape is poor -note this may affect selectivity!

9. Consider UV-Cutoff

10. TEA and TFA degrade and their UV cut-off increases

11. Citrate buffers corrode stainless steel

12. Solubility of salts NH4 < K< Na

Page 32: Mobile Phase Optimization Strategies for Reversed Phase … · Chromatography in a future Essential Guide! When all else fails!! Question and Answer Type your question in the “Submit

Effects of Buffer Concentration on Retention

1. Buffers change the polarity and ionic strength of the mobile phase

2. Doesn’t usually effect analyte retention except where secondary effects are taking place with ionisable analytes (i.e. Silanolinteractions)

3. Beware that some species used as buffers (i.e. TFA) are excellent ion-pairing agents and can drastically alter analyte retention times at the wrong concentration!

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MobilePhase_08.flv

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Working at Low pH with Basic Analytes!

pH 2.5

Amphetamine – peak 7 Amphetamine – peak 7

pH 7.0

Page 35: Mobile Phase Optimization Strategies for Reversed Phase … · Chromatography in a future Essential Guide! When all else fails!! Question and Answer Type your question in the “Submit

Using a sacrificial base

1. Triethylamine (TEA) and Dioctylamine (DOA) can be used to ‘end cap’ the column on the fly

2. Improves peak shape

3. Can be used in conjunction with other buffers at lower concentrations (0.1%)

Page 36: Mobile Phase Optimization Strategies for Reversed Phase … · Chromatography in a future Essential Guide! When all else fails!! Question and Answer Type your question in the “Submit

Using Ion Pair Reagents

1. How do we control retention with amphotericmoleculeswhich cannot be rendered neutral using pH control?

2. Some modern reversed phase HPLC column chemistries are suitable

3. More usual solution is to use ion pairing reagents

4. Ionic / Hydrophobic reagents (e.g. Sodium DodecylSulphonate) are used to ‘pair’ with the analyte ionised moiety in solution

Page 37: Mobile Phase Optimization Strategies for Reversed Phase … · Chromatography in a future Essential Guide! When all else fails!! Question and Answer Type your question in the “Submit

MobilePhase_09.flv

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Using Ion Pair Reagents

1. Actual mechanism is a mixture of ion-pairing and ion-exchange

2. Ion Pair Concentration is important and has an optimum concentration

3. More on Ion Pairing Chromatography in a future Essential Guide!

Page 39: Mobile Phase Optimization Strategies for Reversed Phase … · Chromatography in a future Essential Guide! When all else fails!! Question and Answer Type your question in the “Submit

When all else fails!!

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