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Sunrise HPLC Columns

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Summary

Importance of the topic


Reversed-phase liquid chromatography remains a cornerstone technique in analytical chemistry for separating diverse compounds based on hydrophobic interactions. Control of residual silanol activity on silica-based C18 stationary phases addresses longstanding challenges such as peak tailing and poor retention of basic or polar analytes. The development of silanol activity–controlled (SAC) phases extends chromatographic selectivity by combining hydrophobic, hydrogen-bonding and ion-exchange interactions in one platform.

Objectives and Overview


This application note compares three proprietary reversed-phase columns—Sunrise C30 (triacontyl), C28 (octacosyl) and C18-SAC (silanol activity controlled C18)—to conventional C18 phases. Key goals include evaluating retention behavior for aromatic isomers, basic compounds, vitamins (E and K1), carotenoids, and parabens under varying mobile‐phase compositions, pH and temperature. The study aims to demonstrate enhanced peak shapes, broadened pH range and novel separation modes enabled by selective silanol activity control.

Methodology and Instrumentation


The work employs high‐performance liquid chromatography with UV detection. Columns compared feature different carbon load (14–18 %) and end-capping strategies. Mobile phases include methanol/water, acetonitrile/water or mixtures with buffers (phosphate or ammonium acetate) at pH 2–8. Key instrumentation details:
  • HPLC system with UV detector (250–450 nm)
  • Sunrise series columns: C30, C28 (3 µm/5 µm; 4.6 × 150 or 250 mm), C18-SAC (3 µm/5 µm)
  • Mobile phases: MeOH/H2O, ACN/H2O, ACN/CHCl3, buffered at pH 2.7–7.5
  • Flow rates 0.7–1.0 mL/min; temperatures 15–40 °C

Main Results and Discussion


Sunrise C30 and C28 delivered sharp peaks for isomeric mixtures (BTEX, tocopherols, terphenyls, vitamin K1) that conventional C18 could not resolve, with improved selectivity at lower temperatures. The C18-SAC phase exhibited strong retention and excellent peak shapes for basic analytes (propranolol, nortriptyline, amitriptyline, caffeine) owing to residual silanol–mediated hydrogen‐bonding and ion-exchange interactions. Buffer concentration and pH studies on C18-SAC demonstrated predictable modulation of retention factors (k) via ion‐exchange parameters and ridge‐type elution order for pyridine vs uracil.

Benefits and Practical Applications


  • Enhanced resolution of structural isomers in environmental and pharmaceutical analysis
  • Reduced peak tailing and improved reproducibility for basic and polar compounds
  • Broader operational pH range and robustness under high aqueous conditions
  • Single‐column approach for mixed‐mode separations combining hydrophobic, hydrogen bonding and ion‐exchange mechanisms
  • Scalability from analytical to preparative formats using identical stationary phases

Future Trends and Potential Applications


Further integration of silanol activity control with hybrid silica or core–shell materials could yield next-generation phases offering even higher efficiency and faster separations. Integration with mass spectrometric detection promises enhanced sensitivity for polar/basic analytes. Expanding buffer chemistries and temperature programming may unlock tailored selectivity for emerging complex matrices in metabolomics, peptide analysis and quality control in pharmaceutical manufacturing.

Conclusion


The Sunrise series demonstrates that selective silanol activity control combined with optimized end-capping strategies significantly enhances chromatographic performance across a wide range of analytes. C30/C28 phases excel in isomer separations under high aqueous conditions, whereas C18-SAC provides unique mixed-mode retention for basic and polar compounds. These advances offer robust, versatile solutions for challenging separation tasks in research and industry.

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