Nucleic Acid Quantification

Nucleic Acid Quantification in Microplates

The simplest method for the quantification of nucleic acids uses the intrinsic chromophores provided by the purine and pyrimidine bases which possess a maximum absorptivity at 260 nm. Labware used for this measurement are varied and range from standard 1 cm path length cuvettes to micro-volume analysis where path lengths are typically 20x smaller. The common attribute to these labware is the need to be transparent to this UV light. Many plastics and glass will absorb 260 nm light, hence the widespread use of quartz for these measurements. Microplates are alternative labware, most useful when many samples must be analyzed. Due to their design, the optical path must be perpendicular and pass through the bottom of the wells. Rather than the use of quartz bottoms, microplate manufacturers incorporate UV transparent polymers to allow for the 260 nm measurement. As examples, the table below provides some commonly used microplate options for nucleic acid quantification.

Another consideration in using microplates for nucleic acid quantification is that the path length through the sample will depend on the volume of the solution being measured. Given that most DNA samples will be aqueous in nature, path length correction to 1 cm can be made by measuring the absorbance of water at 977 nm (A977). BioTek's reader control and data analysis software, Gen5, has built-in methods for path length correction to 1 cm for samples in microplates where path length is defined by the volume of the sample added. The calculation is performed by measuring the absorbance peak of water at 977 nm and 900 nm, the difference is then divided by 0.18, which is the absorbance of water at 1 cm, equaling the sample's path length. In the figure below, BioTek's Synergy LX Multi-Mode Reader with absorbance monochromators was used to measure absorbance at 230, 260, 320, 900 and 977 nm in a single protocol to allow automated path length correction and accurate DNA quantification.

Nucleic Acid Purity Assessment

The assessment of the purity of a nucleic acid sample is often performed by a procedure commonly referred to as the A₂₆₀/A₂₈₀ ratio which refers to two spectrophotometric measurements made at these defined wavelengths. Pure nucleic acid samples typically have an A₂₆₀/A₂₈₀ ratio of 2.0. The absorbance of samples that contain a mixture of DNA and protein or other contaminants will be influenced by all molecules present and the ratio will be expected to deviate from the expected ratio. BioTek's range of hybrid microplate readers provide several read options including filter and monochromator based absorbance and fluorescence as well as luminescence measurements over a broad range of sample volumes and vessel types.

For example, spectral analysis for detection of the presence of residual phenol, a commonly used nucleic acid extraction reagent, shows obvious changes in the A₂₆₀/A₂₈₀ ratio as seen in the figure and table below. Thus providing a quick indication of potential contamination.

However, that may not always be the case. For example, in the spectra below, biomolecules were scanned to capture the absorption profiles of biomolecules as well as those of any potential contaminants, should they possess a chromophore of significant absorptivity over this wavelength range. When the A₂₈₀ ratios were plotted against the varying concentrations of DNA/Protein (w/w) it is obvious that the A₂₆₀/A₂₈₀ ratio is reduced with increasing protein contamination. However, note that it takes a significant amount of protein contamination before a meaningful change is noted in the ratio (~40%).

This is also the case for contamination with residual guanadine hydrochloride, a commonly used chaotropic agent, as seen in the figure and table below. While significantly effecting the accuracy of the quantification of DNA the contaminant is not recognizable by examining the ratio alone.

Therefore, it may be prudent to employ a target specific reagent for detection of more complex samples or for validation of upstream processes to insure removal of residual contaminants. For example, by using the dsDNA specific reagent Picogreen in conjunction with fluorescent filters or monochormators an accurate determination of dsDNA concentration can be obtained as seen in the figure below. These determinants than can be compared with absorbance based measurements and any discrepancies can be evaluated for potential causes.

Application Notes

• Fluorometric Quantitation of dsDNA using PicoGreen®(Cytation 1, Cytation 5, Synergy HTX, Synergy Neo2)
• Low-volume, High Throughput Workflow for Analysis of Nucleic Acid Samples for Biobanking (Synergy Neo2)
• Micro-Volume Purity Assessment of Nucleic Acids using A260/A280 Ratio and Spectral Scanning (Epoch 2, Epoch)
• Analytical Performance of a Higher Throughput Micro-Volume Microplate Accessory for Microplate Spectrophotometer Platforms (Epoch 2)
• Micro-Volume PicoGreen® DNA Quantification using BioTek's Take3 Multi-Volume Plate (Synergy HTX)
• Multi-Volume Analysis of Nucleic Acids Using the Epoch Spectrophotometer System (Epoch)
• Low Volume Nucleic Acid Quantification using a Multi-Volume Spectrophotometer System (Epoch)

Visit our Nucleic Acid Quantification application page to see more Nucleic Acid Quantification applications from BioTek instruments.