Protein Concentration Calculator

Our protein concentration calculator determines protein concentration from absorbance at 280nm using the Beer-Lambert Law. This free tool is essential for researchers performing protein quantification, purification, and analysis in molecular biology, biochemistry, and clinical laboratories.

✓ Free to use ✓ Instant results ✓ Multiple protein types ✓ Custom extinction coefficients

Calculate Protein Concentration from A280

Enter absorbance measured at 280nm
Standard cuvettes are 1 cm
Protein Concentration

How to Use This Protein Concentration Calculator

Using this protein concentration calculator is straightforward and takes just seconds. First, measure the absorbance of your protein sample at 280nm using a UV-Vis spectrophotometer. Ensure you’ve blanked the instrument with your buffer solution to get accurate readings. The A280 method is the gold standard for protein quantification because proteins absorb UV light strongly at this wavelength due to aromatic amino acids.

Next, select your protein type from the dropdown menu or choose “Custom Extinction Coefficient” if you know the specific value for your protein. The extinction coefficient (ε) is crucial for accurate calculation, as it varies significantly between different proteins. For example, BSA has an extinction coefficient of 0.667, while lysozyme has 2.64. If you’re unsure, use the generic protein value of 1.0 as an approximation.

Enter your cuvette path length, which is typically 1 cm for standard spectrophotometry cuvettes. Some micro-cuvettes or specialized equipment may use different path lengths, so verify your equipment specifications. The protein concentration calculator will automatically apply the Beer-Lambert Law to determine your sample concentration in mg/mL.

Best Practices for Accurate Measurements

For optimal results with this protein concentration calculator, always ensure your sample is free from particulates by centrifugation or filtration before measurement. Turbidity can significantly affect absorbance readings and lead to overestimation of concentration. Additionally, dilute highly concentrated samples to keep absorbance readings between 0.1 and 1.0, as readings outside this range may be less accurate due to instrument limitations.

Check for nucleic acid contamination by measuring the A260/A280 ratio. Pure protein solutions should have a ratio of approximately 0.57, while ratios above 1.0 indicate significant DNA or RNA contamination that will affect your protein concentration calculator results.

Understanding the Protein Concentration Calculator

The protein concentration calculator is based on spectrophotometric analysis at 280nm, a technique that has been the cornerstone of protein quantification since the 1960s. This method relies on the unique absorbance properties of aromatic amino acids—particularly tryptophan, tyrosine, and to a lesser extent, phenylalanine—which absorb ultraviolet light at 280nm wavelength.

What makes this protein concentration calculator reliable is the direct relationship between absorbance and concentration described by the Beer-Lambert Law. Unlike colorimetric assays that require standard curves and additional reagents, the A280 method provides direct, rapid measurements without sample consumption or chemical modifications. This makes it ideal for valuable samples or when you need to preserve your protein for downstream applications.

The Beer-Lambert Law for Protein Quantification

A = ε × c × l

Rearranged for concentration:
c = A / (ε × l)

where:
A = Absorbance at 280nm (dimensionless)
ε = Extinction coefficient [(mg/mL)^-1 cm^-1]
c = Concentration (mg/mL)
l = Path length (cm)

The extinction coefficient is protein-specific and depends on the number and type of aromatic amino acids in the protein sequence. Proteins rich in tryptophan (like lysozyme) have higher extinction coefficients and absorb more strongly at 280nm, while proteins with few aromatic residues have lower extinction coefficients. This protein concentration calculator accounts for these differences when you select different protein types.

Calculating Molar Concentration

This protein concentration calculator provides results in mg/mL, but you can easily convert to molar concentration (μM or μM) if you know your protein’s molecular weight. Simply divide the mass concentration by molecular weight (in kDa) to get mM, then multiply by 1000 for μM. For example, if the protein concentration calculator shows 1.5 mg/mL and your protein is 50 kDa, the molar concentration is 30 μM.

Practical Examples Using the Protein Concentration Calculator

Example 1: BSA Protein Quantification

Scenario: A researcher purified bovine serum albumin (BSA) and needs to determine its concentration for downstream experiments.

Measurements:

  • A280 absorbance: 0.450
  • Protein type: BSA (ε = 0.667)
  • Path length: 1 cm

Using the protein concentration calculator:

c = 0.450 / (0.667 × 1) = 0.675 mg/mL

Result: The BSA concentration is 0.675 mg/mL or 675 μg/mL, which is ideal for most biochemical assays.

Example 2: Antibody (IgG) Concentration for ELISA

Scenario: An immunologist needs to determine antibody concentration for ELISA plate coating.

Measurements:

  • A280 absorbance: 1.104
  • Protein type: IgG (ε = 1.38)
  • Path length: 1 cm

Using this protein concentration calculator:

c = 1.104 / (1.38 × 1) = 0.800 mg/mL

Result: The IgG concentration is 0.8 mg/mL. For ELISA coating, this would typically be diluted to 1-10 μg/mL.

Example 3: Enzyme Preparation with Custom Extinction Coefficient

Scenario: A biochemist purified a recombinant enzyme with a calculated extinction coefficient of 1.52 (mg/mL)^-1 cm^-1.

Measurements:

  • A280 absorbance: 0.912
  • Custom extinction coefficient: 1.52
  • Path length: 1 cm

Using the protein concentration calculator:

c = 0.912 / (1.52 × 1) = 0.600 mg/mL

Result: The enzyme concentration is 0.6 mg/mL, suitable for activity assays and crystallization trials.

Factors Affecting Protein Concentration Measurements

While the protein concentration calculator provides accurate results under optimal conditions, several factors can influence measurement accuracy. Understanding these variables helps ensure reliable quantification for your research applications.

Sample Purity and Contaminants

Nucleic acid contamination is the most common source of error when using a protein concentration calculator. DNA and RNA absorb strongly at 260nm but also contribute to absorbance at 280nm. A pure protein sample should have an A260/A280 ratio of approximately 0.57. Ratios above 1.0 indicate significant nucleic acid contamination, which will cause the protein concentration calculator to overestimate protein levels. In such cases, consider using alternative methods like Bradford or BCA assays, or remove contaminants through additional purification steps.

Buffer Components and pH Effects

The extinction coefficient used in this protein concentration calculator is pH-dependent, as the ionization state of aromatic amino acids affects their absorbance properties. Measurements should be performed at physiological pH (7.0-7.5) for standard extinction coefficients to be valid. Additionally, some buffer components can interfere with A280 measurements. Avoid using reducing agents like DTT or β-mercaptoethanol at high concentrations, as they absorb in the UV range.

Sample Turbidity and Light Scattering

Protein aggregates, precipitates, or particulate matter cause light scattering that adds to measured absorbance, leading to inflated results from the protein concentration calculator. Always centrifuge samples at high speed (12,000-15,000 × g) for 10 minutes before measurement, or filter through 0.22 μm filters to remove particles.

Applications in Research and Industry

Researchers use this protein concentration calculator across diverse applications: preparing samples for SDS-PAGE, western blotting, mass spectrometry, structural biology studies, enzyme kinetics, and therapeutic protein development. In biopharmaceutical manufacturing, accurate protein quantification is critical for formulation and quality control, making this protein concentration calculator an essential tool in GMP laboratories.

Frequently Asked Questions

What is a protein concentration calculator?
A protein concentration calculator is a tool that determines protein concentration in a sample using absorbance at 280nm (A280). It applies the Beer-Lambert Law with protein-specific extinction coefficients to convert absorbance readings into concentration values in mg/mL or μM. This method is rapid, non-destructive, and requires minimal sample volume.
How accurate is the A280 method for protein concentration?
The A280 method is highly accurate for purified proteins, typically within 5-10% accuracy when using correct extinction coefficients. However, accuracy depends on several factors: knowing the correct extinction coefficient for your specific protein, sample purity (absence of nucleic acid contamination), and proper instrument calibration. For highly accurate work, verify results using alternative methods like amino acid analysis.
What extinction coefficient should I use?
Use protein-specific extinction coefficients when available from published data or calculate from amino acid composition using tools like ExPASy ProtParam. Common values: BSA (0.667), IgG (1.38), Lysozyme (2.64), Hemoglobin (1.03). For unknown proteins, use a generic value of 1.0 (mg/mL)^-1 cm^-1 as an approximation, though this may introduce 20-30% error.
Why use 280nm wavelength for protein measurement?
Proteins absorb strongly at 280nm due to aromatic amino acids (tryptophan, tyrosine, and phenylalanine). Tryptophan has the highest extinction coefficient at 280nm, followed by tyrosine. This wavelength provides excellent sensitivity for most proteins while minimizing interference from buffer components, peptide bonds, and other common laboratory chemicals.
Can this calculator measure protein molar concentration?
Yes, this protein concentration calculator can help you determine molar concentration (μM) if you know the molecular weight. The calculator provides mass concentration in mg/mL. To convert to molar: divide by molecular weight (in kDa) to get mM, then multiply by 1000 for μM. Example: 1.5 mg/mL of a 50 kDa protein equals 30 μM.
What affects protein concentration measurements at A280?
Several factors affect accuracy: nucleic acid contamination (DNA/RNA absorb at 260-280nm causing overestimation), sample turbidity from aggregates or particles, buffer composition and pH, protein aggregation state, disulfide bond status, instrument wavelength accuracy, and cuvette cleanliness. Always blank with appropriate buffer and verify sample clarity before measurement.
How do I use this protein concentration calculator?
Enter your A280 absorbance reading from the spectrophotometer, select your protein type from the dropdown (or enter a custom extinction coefficient), specify the cuvette path length (usually 1 cm), and click Calculate. The protein concentration calculator instantly provides concentration in mg/mL using the Beer-Lambert Law. For best results, ensure samples are clear and properly blanked.
What is the Beer-Lambert Law for proteins?
The Beer-Lambert Law states that absorbance (A) is directly proportional to concentration (c), extinction coefficient (ε), and path length (l): A = ε × c × l. For protein concentration calculations, we rearrange this to: c = A / (ε × l). This fundamental relationship allows direct determination of protein concentration from absorbance measurements without requiring standard curves or additional reagents.
Is this calculator free to use?
Yes, this protein concentration calculator is completely free to use with no registration required. Access it unlimited times on any device. We provide this tool as a resource for the scientific community to support protein research and biochemical analysis worldwide.
What’s the difference between A280 and Bradford/BCA methods?
A280 (used by this protein concentration calculator) is direct, rapid, and non-destructive but requires pure protein and knowing the extinction coefficient. Bradford and BCA are colorimetric assays that work with crude samples and don’t need extinction coefficients, but they require reagents, standard curves, consume sample, and can be affected by detergents and reducing agents. Choose A280 for pure proteins and quick measurements.

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Sources and References

This protein concentration calculator is based on established spectrophotometric principles and standard laboratory protocols. The extinction coefficients and formulas are derived from peer-reviewed scientific literature and authoritative biochemistry resources.