Beer Lambert Law Calculator
Dimensionless value between 0 and 4
Beer Lambert Law: Understanding Spectroscopic Concentration Calculations
What is Beer Lambert Law?
Beer Lambert Law (also known as Beer’s Law or the Beer-Lambert-Bouguer Law) is a fundamental principle in spectroscopy that describes how light is absorbed as it passes through a medium containing absorbing species. This law is crucial for determining the concentration of substances in solution by measuring their absorbance at specific wavelengths.
The law is particularly important for chemists, biochemists, pharmaceutical researchers, and analytical scientists who need to quantify substances in various samples. It provides a direct relationship between the concentration of a substance and the amount of light it absorbs, making it possible to determine unknown concentrations from measured absorbance values.
Common misconceptions about Beer Lambert Law include confusing absorbance with transmittance, misunderstanding the relationship between path length and concentration, and incorrectly assuming that the law applies to all types of light sources or wavelengths. The law specifically applies to monochromatic light and dilute solutions.
Beer Lambert Law Formula and Explanation
Where:
| Variable | Meaning | Unit | Typical Range |
|---|---|---|---|
| A | Absorbance | Dimensionless | 0 to 4 |
| ε | Molar Extinction Coefficient | M⁻¹cm⁻¹ | 1000 to 100000 |
| b | Path Length | cm | 0.1 to 10 |
| C | Concentration | M (Molarity) | 0.001 to 1 |
The formula can be rearranged to solve for concentration:
This rearranged formula is what our calculator uses to determine the concentration of a substance when the absorbance, path length, and molar extinction coefficient are known.
Practical Examples
Example 1: Protein Concentration Analysis
Inputs:
- Absorbance (A): 0.8
- Path Length (b): 1.0 cm
- Molar Extinction Coefficient (ε): 14,000 M⁻¹cm⁻¹ (for proteins at 280 nm)
Calculation:
C = 0.8 / (14,000 × 1.0) = 5.71 × 10⁻⁵ M
Result: The protein concentration is 57.1 μM (micromolar)
Example 2: DNA Quantification
Inputs:
- Absorbance (A): 1.2
- Path Length (b): 1.0 cm
- Molar Extinction Coefficient (ε): 50,000 M⁻¹cm⁻¹ (for DNA at 260 nm)
Calculation:
C = 1.2 / (50,000 × 1.0) = 2.4 × 10⁻⁵ M
Result: The DNA concentration is 24 μM (micromolar)
How to Use This Beer Lambert Law Calculator
Using our Beer Lambert Law calculator is straightforward:
- Enter the absorbance value measured from your spectrophotometer. This should be a dimensionless value between 0 and 4.
- Set the path length of your cuvette in the appropriate units (cm, mm, or m). Standard cuvettes typically have a path length of 1 cm.
- Input the molar extinction coefficient for your substance at the specific wavelength used. This value is typically found in literature or can be determined experimentally.
- Click “Calculate Concentration” to get your result.
- Review the results and copy them if needed for your records.
When selecting units, ensure consistency between your path length and molar extinction coefficient units. If your path length is in millimeters, use the M⁻¹mm⁻¹ unit for the molar extinction coefficient.
Key Factors That Affect Beer Lambert Law Calculations
- Wavelength Selection – The molar extinction coefficient varies with wavelength, so measurements must be made at the specific wavelength where the substance has maximum absorbance.
- Solution Concentration – The law applies best to dilute solutions. At high concentrations, deviations may occur due to molecular interactions.
- Temperature – Temperature changes can affect both the molar extinction coefficient and the physical properties of the solution.
- Path Length – Longer path lengths increase absorbance proportionally, affecting the calculated concentration.
- Sample Purity – Impurities can contribute to absorbance at the measurement wavelength, leading to inaccurate concentration calculations.
- Light Source Quality – The law assumes monochromatic light. Polychromatic light can cause deviations from the linear relationship.
Frequently Asked Questions