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Overcoming Peak Tailing of Basic Analytes: Silica Type A Stationary Phases RP

HPLC/UHPLC Technical Tip
Level: Basic

In this technical tip, we will address the common issue of peak tailing encountered when working with basic analytes and “type A” silicas and offer two strategies to overcome it.

Introduction

Early reversed phase columns were based on “type A” silicas, these materials had substantial metal contamination, causing the silanol groups on the surface of the silica to have greater and more variable activity. Manufacturers endcapped the materials as far as possible after bonding with C18 reagents, in an attempt to reduce the number of sites where ion exchange could take place. However basic compounds would generally tail badly. Let’s explore how we can overcome this limitation.

Strategies for peak shape improvement

These strategies will help diminish the tailing effect but may not completely remove it as demonstrated in the below example chromatograms (Figure A and B).

tech tips figure

Mobile Phase
20 mM potassium phosphate buffer pH= 2.5 : Methanol (70:30)
Flow Rate
1 mL/min
Detection
UV-Vis @254 nm

tech tips figure

Mobile Phase
20 mM potassium phosphate buffer pH= 3 with 400uL/L Triethylamine : Acetonitrile (63:37)
Flow Rate
1 mL/min
Detection
UV-Vis @230 nm

Figure A shows the moderate effect of using an acidic pH to mitigate tailing for benzylamine, while Figure B shows the resulting chromatography after adding triethylamine as a modifier.

We recommend the use of type B (ultra-pure) silica in the development of new separations. Luna™ Omega fully porous and Kinetex™ Core-Shell columns provide excellent peak shape for challenging compounds.

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