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Quantitative Determination of Peptides by Sulfhydryl (-SH) Groups

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Quantitative Determination of Peptides by Sulfhydryl (-SH) Groups

Author: David Van Horn, Greg Bulaj
Source: Contributed by David Van Horn, Dept. of Chemistry, UC Berkeley Greg Bulaj, Dept. of Biology, University of Utah
Abstract: This is the standard �llman� Test?for the determination of free thiols. It works well for small peptides and proteins synthesized using standard solid phase synthetic methods.

Overview

 

 

This is the standard “Ellman’s Test” for the determination of free thiols. (Ref. 1)  It works well for small peptides and proteins synthesized using standard solid phase synthetic methods.  Peptides from these syntheses are usually in their reduced form, and are usually stable to oxidation in acidic solutions.  Free thiol can be determined in solutions collected from chromatographic separations or from reconstituted lyophilized samples.  This protocol has been used for peptides (3 to 26mer) with a single Cys residue present and lacking tryptophan. (Ref. 2, 3)  The technique should be feasible for multiple Cys residues (Hint 5).

 

 

Procedure

 

 

  1. Turn on UV-Vis spectrophotometer and setup, in your notebook, the Table described below.

     

  2. In an appropriate cuvette (see Hint 1), add 50 µ L of the DTNB solution, 100 µ L Tris solution, and water up to (1000 µ L - sample µ L).

     

  3. Volume example:       50 DTNB
                                  100 Tris
                                  840 Water
                                  990  µ L initial volume (take blank)
                                  + 10 Sample (added via syringe!)
                                  1000 µ L final volume (take reading at 412 nm)

     

  4. Mix solution carefully using pipette.  Place cuvette into UV-Vis spectrophotometer and take a background scan using the solution as background.

     

  5. Introduce sample solution into cuvette with a syringe (Hint 2), keeping the cuvette in the instrument (Hint 3).

     

  6. Carefully mix solution with a pipettemen without disturbing the cuvette.

     

  7. Scan sample and record Absorbance at 412 nm. (Hint 4)

     

  8. Calculate absorbance for each sample and then average the results, divide this by 13600 M-1 cm-1 (the extinction coefficient of the reagent) to get the molarity of the solution. (Hint 5)

     

  Sample Table and Calculation (Volumes in µ L):

 

 

 

 

DTNB

 

 

Tris

 

 

Water

 

 

Sample

 

 

Abs (412nm)

 

 

Abs (sample)

 

 

 

 

 

 

 

 

 

 

 

 

 

 

50

 

 

100

 

 

840

 

 

10

 

 

0.5010

 

 

50.1

 

 

50

 

 

100

 

 

835

 

 

15

 

 

0.7540

 

 

50.3

 

 

50

 

 

100

 

 

830

 

 

20

 

 

1.0080

 

 

50.4

 

 

 

 

 

Equation:

 

 

Abs(sample) = (Tot. Vol./sample vol.) x (Abs 412 )

 

 

Sample Calculation:          Ave. = 50.2/13600 = 3.7 mM thiol

 

 

  Solutions

 

  DTNB solution          =          50 mM sodium acetate (NaOAc)

 

   2 mM DTNB in H2 O

 

 

     (refrigerate)

 

 

  TRIS solution          =            1 M Tris / pH 8.0

 

 

 

 

Biochemicals  

 

DTNB = Ellman’s reagent = 5,5’-Dithiobis(2-nitrobenzoic acid)

 

 

Protocol Hints

 

 

  1.   1 mL disposable plastic cuvettes work well. (However, see Hint 3)

     

  2. Keep samples frozen until use and on ice.  Since this is supposed to be quantitative, we recommend using a syringe, not a pipette, for the sample solution, especially for small volumes and dilute solutions.

     

  3. When using plastic cuvettes, our experience has been that removal and reintroduction into the instrument of the same or different cuvette leads to anomalous readings/data.  Thus, careful technique is used to introduce the sample and mix it in the sample holder of the instrument.  Quartz cuvettes have no such problem with this. (But you have to clean them up each use.)

     

  4.   If you set up the cuvettes and sample on ice near the UV-Vis, you can minimize the time the determinations take.  Also, you won’t be accused of monopolizing the instrument.

     

  5. The calculation is for total free thiol.  Presumably you know beforehand the total number of thiols are in your peptide.  Divide the determined concentration by the number of thiols, and this is the peptide concentration. (See Hint 6)

     

  6. If your peptide contains more than 4 cysteine residues, you may want to recalculate the excess of DTNB and use a greater amount (e.g. 75 or 100 µ L of solution)

     

  References

 

  1.   Ellman, G. L. (1959)  Arch. Biochem. Biophys. 82 , 70-77.  (Original determination)

     

  2.   Bulaj, G.; Kortemme, T.; Goldenberg, D. P.  (1998)  Biochemistry  37 , 8965-8972.  (Recent usage)

     

  3.   Van Horn, J. D.; Bulaj, G.; Burrows, C. J.  (2001)  Unpublished results.

     

 

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