Protein Detection and Quantitation (BIOC3570 F24 02) PDF

Summary

These lecture notes cover protein detection and quantitation, focusing on colorimetric assays. They detail applications and analytical challenges, including the 2008 Chinese milk scandal, and discuss various techniques like UV spectrophotometry and the Bradford/BCA assays.

Full Transcript

# Protein detection and quantitation (1) ## Colorimetric Assays ### Protein quantitation: applications - Quantification of protein in foods (protein content is noted on all food labels) - Medical diagnosis: e.g., measurement of total protein in urine is important for diagnosing kidney dysfunction...

# Protein detection and quantitation (1) ## Colorimetric Assays ### Protein quantitation: applications - Quantification of protein in foods (protein content is noted on all food labels) - Medical diagnosis: e.g., measurement of total protein in urine is important for diagnosing kidney dysfunction (proteinuria) - Protein therapeutics need exact quantitation of dosage, e.g., insulin, HGH, therapeutic antibodies. - Biochemistry/molecular biology reagents. - Protein biochemistry applications require accurate protein quantitation (e.g., activity measurements are proportional to protein quantity) ### Protein quantitation: Analytical challenges - Proteins are challenging reagents to quantify because: - Each protein has a unique amino acid composition. - Unless the detection method is equally sensitive to all residues, quantitation will be inaccurate unless corrected for composition. - Non-peptide components (e.g., glycosylation, co-factors) can contribute to protein mass (and possibly signal). - Proteins can show microheterogeneity (e.g., apo- vs holoproteins, splice variants, alleles, variable glycosylation). - Highly purified reference materials are generally not available. - Diverse excipients are usually present in the same solution - e.g., buffers, detergents, reducing agents, salts etc. ### Deliberate, criminal efforts to subvert analysis - The 2008 Chinese milk scandal was a food safety incident in China. - The assays that test protein levels in food products essentially measure organic nitrogen. - Milk and infant formula can be made cheaper by removing protein, so this is monitored. - Some "enterprising" Chinese companies started adding melamine to baby formula and milk to add back missing nitrogen. - Melamine causes kidney stones and other kidney damage. - China reported an estimated 300,000 victims - An estimated 54,000 babies were hospitalized, and 11 infants died. ### Protein quantification - common techniques - Total nitrogen content. - Gravimetry. - Hydrolysis -> amino acid analysis. - UV spectrophotometry (A280). - Colorimetric assays: - BCA. - Bradford. ### Bulk methods for food analysis - Estimate protein content of complex biological materials ### Research labs - More accurate protein amount from pure samples. ### Protein quantitation by UV absorbance (A280) - Some amino acids absorb light at 11 = 280 nm, this can be used to quantify proteins. - However, many other analytes (e.g., DNA) absorb UV light, causing potential false positive signals. - UV quantitation is only applicable to relatively pure protein samples. - You need to know the protein sequence to predict the absorbance accuracy. - However, under the right conditions, UV absorbance can achieve **much better accuracy** than the Bradford or BCA assays. - We will discuss this method later in the course as part of UV-vis spectroscopy ### Chromogenic assays in biochemistry - Many analytes of interest (including polypeptides and most proteins) do not absorb visible light. - However, we can exploit chemical reactions that will generate substances that do. - These are called "colorimetric" or "chromogenic" assays. - Most of the common protein assays work this way. ### Colorimetric Chromogenic assays in biochemistry - Colorimetric assays have also been developed for many other classes of biomolecules, e.g.: | Analyte | Reagent | |---|---| | Amine groups (Lys, N-term) | ninhydrin | | DNA | diphenylamine | | RNA | Bial's reagent | | Thiols (cysteine, CoA) | Ellman's reagent | | Glucose | glucose oxidase/peroxidase system | ### Triarylmethane Dyes - Triaryl methane dyes share a common core structure. - These molecules have an intense blue or purple colour. - Gram stain which labels the peptidoglycan of bacteria is an important reagent in this molecular class. ### Triaryl methane dyes: colour shifts - These molecules have a triphenyl methane group with a ternary amine at the p-position. - The amines will accept protonation in a pH-dependent manner. - The change in the electronic structure causes a color change. - The non-polar triphenyl readily binds non-polar surfaces. - Importantly, the pKa is shifted in a non-polar environment. ### Coomassie Blue (synthetic triarylmethane dye) - Coomassie is a modified version of the basic triarylmethane structure (note the additional sulfophenyl and phenolic groups). - Originally, Coomassie blue waS invented as a wool dye (keratin is a protein). - Biochemists found it worked well as a protein stain (see electrophoresis), and later adopted it for protein quantitation. ### Coomassie binds the hydrophobic interior of acid unfolded proteins. - The protein should have been unfolded due to excess acid/increase in pH as Coomassie needs to be protonated. - **Protonation**: Phosphoric acid protonates free coomassie which is then red-brown in colour. Acid denatures the protein. - **Denaturation**: Coomassie binds in the exposed, hydrophobic protein interior. pKa is shifted towards neutral. Coomassie loses proton(s). Protein bound coomassie is blue-purple. ### Bradford dye-binding assay - Coomassie Blue has two SO groups, making it anionic. - Under acidic conditions (8.5% phosphoric acid), dye binds to protein (especially to basic and aromatic a.a. residues). - Note: the protein is acid denatured under these conditions. - Binding shifts the protonation equilibrium of dye towards less-protonated forms (protein environment shifts the pKa). - This shifts the colour from red-brown to blue. - The degree of colour shift is directly proportional to the amount of protein. ### Bradford assay: running the assay - A dilution series of a standard protein (often bovine serum albumin) of known concentration is prepared. - These standard samples, as well as the unknown protein samples are then mixed with the assay reagent. - After incubation, the absorbance is measured using a spectrophotometer. - Absorbance is typically measured at 595 nm, the peak absorbance of the anionic (blue) species. - The standard samples are used to prepare a standard curve. - Sample protein concentrations are determined by comparing their assay responses to the standard curve. ### Protein assays: Data - Net absorbance is plotted against protein concentration for the protein standard (here BSA). - Protein concentration for the sample is read by reading the BSA concentration that gives the measured absorbance. - Note that the fit (red line) is only linear to ~700 g/ml. ### Assays: Dynamic - Any assay can be applied only within a certain dynamic range. - Test several dilutions of your sample. - Rely only on the results that are within the linear dynamic range of the assay. ### BSA: experimental accuracy and precision - Bradford assays are quite reproducible with good technique. - However, the Bradford assay response varies a great deal with different proteins. - Bradford is more sensitive to hydrophobic and basic residues. - Since you do not know a priori how a specific protein will respond this reduces the accuracy of the assay. - The accuracy of the Bradford assay is only ~± 20%. ### Bradford assay - limitations and uses - The Bradford assay is compatible with most common biochemical reagents - e.g., salts, chelators, reducing agents. - However, detergents will also bind the Coomassie dye, and give a false positive result. - The accuracy of this assay is also somewhat limited, and the dynamic range not great. - However, it is quick, cheap and easy, needs only standard lab equipment (spectrophotometer) and works well for measuring total protein concentrations (e.g., during a purification). ### BCA assay - BCA reagent solution contains BCA and CuSO4 at pH 11.25. - **Step 1**: protein reduces Cu2+ to Cu+. - **Step 2**: selective detection of Cu⁺ by BCA reagent results in a purple color. ### BCA assay - chemistry - Cysteine, Tyrosine and Tryptophan side chains react with copper, reducing it. - Copper is also reduced by the Biuret reaction with the peptide backbone. - The assay therefore detects all proteins, but is more sensitive to Tyr, Trp and Cys -rich proteins. ### The Chelate effect - In chelation a single ligand ligates a metal ion at multiple positions simultaneously. - Ligands pay an entropic cost (loss of conformational freedom) when binding a metal. - **Keq** is 109-fold more favourable for formation of the chelate complex, so a second ligand within the same complex is much lower entropic cost. More binding sites and a more rigid chelator enhance this effect for even tighter binding. ### Chelates (examples in biochemistry) - In nature: heme: porphyrin-iron chelate. - In the lab: EDTA: transition-metal scavenger. ### Bicinchoninic acid (BCA): - BCA: a sensitive, stable, and highly specific chelating ligand for Cu+. - **Cu++:** dº; prefers 5- or 6-coordinate square-planar geometry. - **Cu+: ** d¹º; prefers 4-coordinate tetrahedral geometry. ### BCA assay procedure - The basic procedure of the BCA assay is similar to the Bradford assay. - The reactions need to be heated as the Biuret reaction is inefficient at room temperature. - Heating to 60°C instead of 37°C will increase colour development roughly 8-fold - so much more sensitive. - Absorbance is measured at 562 nm (the colour is different than the Bradford assay). ### BCA assay - limitations and uses - The BCA assay is fast, reproducible, inexpensive and relies only on standard lab equipment. - **Reducing agents** will reduce Cu+, giving a false positive signal. - **Chelators** (e.g., EDTA) will compete with BCA for Cu+, weakening the signal (false negative). - Most other standard reagents, including detergents are compatible. - Because of the composition dependence, the BCA assay shows protein-to-protein variation, but less so than the Bradford assay. ### Colorimetric protein assays: summary - **Principle**: Protein reacts with reagents to give coloured complex. - **Application**: Quantitation of protein content in sample. **Strengths:** - **Little instrumentation required** (plate reader or spec). - **Good for comparing similar batches**, e.g., lysates of cells treated in an experiment. - **E.g., normalizing inputs for gels or western blots**. **Weaknesses:** - **Indirect assay**: absolute quantitation is poor (so not ideal if you need absolute enzyme concentration to figure out a kcat). - **Subject** to interferences from reagents. - **Limited dynamic range**.

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