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Open AccessJournal ArticleDOI

Interaction of Proteins with Sulfide

Doriano Cavallini, +2 more
- 01 May 1970 - 
- Vol. 14, Iss: 1, pp 169-174
TLDR
The addition of sodium sulfide to disulfide-containing proteins dissolved in 0.01 N NaOH produces an absorption in the range of 320–350 nm similar to that exhibited by cystine or cystamine treated under the same conditions.
Abstract
The addition of sodium sulfide to disulfide-containing proteins dissolved in 0.01 N NaOH produces an absorption in the range of 320–350 nm similar to that exhibited by cystine or cystamine treated under the same conditions. Proteins free of cystine and cysteine and proteins containing disulfide bonds which have been reduced with sodium borohydride do not produce this absorbance. Urea and guanidine at 6 M concentration increase the rate of production of the absorbance while sodium dodecyl sulfate at concentration of 0.02 M has an inhibitory effect both on the rate and the extent of the absorbance. The effect of pH, concentration of reagents and of the additions of cyanide and hypotaurine has been studied. The 320–350 nm absorbance as been related to the production of persulfide groups (R-SSH) as a result of the cleavage of disulfide bonds by sulfide. Attempts to prepare a purified model protein containing persulfide groups have failed owing to the instability of the persulfide group in conditions far from those used for its preparation.

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Citations
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References
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Journal ArticleDOI

A micro biuret method for protein determination; determination of total protein in cerebrospinal fluid.

TL;DR: A rapid and convenient colorimetric method for the determination of small amounts of protein, based on the biuret reaction and readings at 330 mμ, is described.
Journal ArticleDOI

Determination of Disulphide Groups in Proteins

TL;DR: This communication deals with the method recently used in the laboratory for the determination of disulphide groups using sodium borohydride (NaBH4) in 8 molar urea as reducing agent and 5,5′-dithiobis (2-nitrobenzoic) acid (DTNB) as a thiol disulPHide exchanger.
Journal ArticleDOI

The content and possible catalytic significance of labile sulfide in some metalloflavoproteins.

TL;DR: Evidence is presented which suggests that in liver santhine oxidase the labile sulfide is linked to the protein through ferric iron and another sulfur atom, and this possibility was provided by the results of investigations of the ferredoxins.
Journal ArticleDOI

Iron-sulphur proteins.

TL;DR: These electron transfer agents often have unusually low redox potentials as discussed by the authors, and are involved in nitrogen fixation as well as photosynthesis, and are known from higher plants and bacteria.
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