Over the past decade, high-performance liquid chromatography (HPLC) has increasingly replaced spectroscopic methods and gas chromatography (GC) in both quantitative and qualitative drug analysis. Initially seen as complementary to gas chromatography, HPLC has now largely supplanted itself in pharmaceutical analysis due to its versatility, including the ability to adjust mobile phase polarity and select stationary phases tailored to specific substances.
High-performance liquid chromatography is a powerful analytical technique used to separate, identify, and quantify each component in a mixture. It is widely employed in various fields, such as pharmaceuticals, environmental monitoring, food and beverage analysis, and chemical research.
HPLC operates by passing a liquid sample through a column packed with solid adsorbent material under high pressure, enabling the separation of compounds based on their different interactions with the stationary phase.
Common LC Column Formats
Nano LC Columns
High powered sensitivity for exceedingly small samples (Column ID 50-75 μm)
Micro LC Columns
Increased sensitivity for small samples (Column ID 0.15-.05 mm)
UHPLC Columns
High speed separations of analytes (Column ID 1.0-2.1 mm)
Analytical LC Columns
General, all-purpose separations (Column ID 2.1-4.6 mm)
Semi-Prep and Preparative LC Columns
Large scale isolation and purifications (7.8-100 mm)
HPLC columns are critical components in the HPLC system, responsible for the actual separation of the sample components. These columns are typically made of stainless steel and packed with tiny, uniform particles known as the stationary phase. The choice of stationary phase material and the column's dimensions (length, diameter, and particle size) significantly influence the separation process and the efficiency of the analysis. Coupled with sensitive detector systems, HPLC has become a widely employed method for confirming drug identity, providing quantitative results, and monitoring therapeutic progress in disease management.
High-pressure liquid chromatography (HPLC) is a technique that uses a solid stationary phase and a liquid mobile phase (e.g., acetonitrile, methanol, phosphate buffer, etc.) to separate components in a mixture. In the HPLC setup, the stationary phase is often housed in specialized columns, commonly referred to as HPLC columns, which are typically constructed from high-quality stainless steel. Liquid chromatography columns in HPLC are designed to withstand the high pressures required for efficient separation. Chemical interactions between the stationary phase and the chemical composition of the components in the mixture result in the components traveling at different speeds in the HPLC column and separating or eluting at different times from the column stationary phase.
The analytical column in HPLC serves as the heart of the chromatographic system. HPLC columns come in various dimensions and particle sizes, catering to different analytical needs and the nature of the compounds being separated. The different types of HPLC columns are described below:
Columns in normal-phase HPLC have a polar stationary phase and a non-polar mobile phase. They are suitable for separating polar compounds or those with functional groups that interact favorably with the polar stationary phase.
Reversed-phase HPLC columns feature a non-polar stationary phase and a polar mobile phase. They are widely used for separating non-polar and moderately polar compounds.
Anion exchange columns retain negatively charged ions. They are employed for separating anions based on their charge and size.
Size-exclusion chromatography (SEC) columns separate analytes based on their size. Larger molecules elute first as they pass through pores in the stationary phase, while smaller molecules are retained longer.
Hydrophilic Interaction Liquid Chromatography (HILIC) columns retain polar compounds using a hydrophilic stationary phase and an HPLC mobile phase containing a high percentage of organic solvent.
Choosing the correct HPLC column is essential for achieving optimal separation and analysis of compounds. Several factors need to be considered when selecting a column for HPLC:
Columns for HPLC are key components that facilitate the separation of analytes in chromatographic analysis. These analytical columns in HPLC contain a stationary phase, which interacts with the sample components as they pass through the column under high pressure. Choosing the column type and conditions is crucial for achieving efficient and selective separation of analytes in HPLC analysis.
Fully porous particles are the traditional particles used in HPLC columns. These particles have pores that allow the mobile phase and analytes to diffuse throughout the entire particle. This leads to a high surface area, enabling good separation efficiency. Fully porous particles are versatile and are often applied in a wide range of analytical applications, particularly when high resolution is required.
Superficially porous particles, also known as core-shell particles, consist of a solid, non-porous core surrounded by a thin, porous layer. This unique design reduces the diffusion path of analytes, leading to faster separations with high efficiency, often comparable to sub-2 micron particles but with the advantage of lower back pressure. These particles are ideal for applications requiring rapid analysis without compromising the resolution.
Monolithic particles are made from a continuous porous rod rather than packed particles. This structure offers high permeability, which allows for faster flow rates with lower back pressure. Monolithic columns are known for their robustness and are particularly effective in handling complex matrices. They are well-suited for high-speed separations and are often used in bioanalytical applications, such as the analysis of proteins and peptides.
Sub-2-micron particles are extremely small, providing a very high surface area that results in high efficiency during separations. These particles are commonly used in Ultra-High Performance Liquid Chromatography (UHPLC), a technique that operates at higher pressures to achieve faster and more efficient separations. Sub-2-micron particles are ideal when the highest possible resolution and speed are required, particularly in complex separations involving closely related compounds.
Silica-based particles are the most commonly used stationary phases in HPLC due to their mechanical strength, chemical stability, and compatibility with various modifications, such as bonded phases. These particles can be fully porous or superficially porous and are available in various particle sizes. Silica-based particles are used in a wide range of HPLC applications where chemical stability and mechanical strength are essential.