Cyanogen bromide

Cyanogen bromide
Names
Preferred IUPAC name
Carbononitridic bromide[1]
Systematic IUPAC name
Bromidonitridocarbon
Other names
  • Bromine cyanide[2]
  • Bromocyan
  • Bromocyanide
  • Bromocyanogen
  • Campilit
  • Cyanobromane
  • Cyanobromide
Identifiers
Abbreviations CB
1697296
506-68-3 Yes
ChemSpider 10044 Yes
EC number 208-051-2
Jmol-3D images Image
MeSH Cyanogen+Bromide
PubChem 10476
RTECS number GT2100000
UN number 1889
Properties
CBrN
Molar mass 105.921 g mol1−
Appearance Colorless crystals
Density 2.015 g mL−1
Melting point 50 °C (122 °F; 323 K)
Boiling point 61 °C (142 °F; 334 K)
Reacts
Vapor pressure 16.2 kPa
Thermochemistry
Std enthalpy of
formation (ΔfHo298)
136.1–144.7 kJ mol−1
Hazards
GHS pictograms
GHS signal word DANGER
H300, H310, H314, H330, H410
P260, P273, P280, P284, P302+350
EU classification T+ N
R-phrases R26/27/28, R34, R50/53
S-phrases S36/37/39, S45
NFPA 704
Flammability code 0: Will not burn. E.g., water Health code 4: Very short exposure could cause death or major residual injury. E.g., VX gas Reactivity code 1: Normally stable, but can become unstable at elevated temperatures and pressures. E.g., calcium Special hazards (white): no codeNFPA 704 four-colored diamond
0
4
1
US health exposure limits (NIOSH):
5 mg m−3
Related compounds
Related alkanenitriles
Except where noted otherwise, data is given for materials in their standard state (at 25 °C (77 °F), 100 kPa)
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Infobox references

Cyanogen bromide is a pseudohalogen compound with the formula CBrN. It is a colorless solid that is widely used to modify biopolymers, fragment proteins and peptides, and synthesize other compounds.

Synthesis, basic properties, and structure

The carbon atom in cyanogen bromide is bonded to bromine by a single bond and to nitrogen by a triple bond (i.e. BrC≡N). The compound is linear and quite polar, but it does not spontaneously ionize in water. Therefore, it dissolves in both water and polar organic solvents.

Cyanogen bromide can be prepared by oxidation of sodium cyanide with bromine, which proceeds in two steps via the intermediate cyanogen ((CN)2 or N≡CC≡N).

2 NaCN + Br2 → (CN)2 + 2 NaBr
(CN)2 + Br2 → 2 BrCN

Cyanogen bromide is hydrolyzed by water to release hydrogen cyanide and hypobromous acid

BrCN + H2O → HCN + HOBr

Biochemical applications

The main uses of cyanogen bromide are to immobilize proteins, fragment proteins by cleaving peptide bonds, and synthesize cyanamides and other molecules.

Cyanogen bromide activation method

Protein immobilization

Cyanogen bromide is often used to immobilize proteins by coupling them to reagents such as agarose for affinity chromatography.[3] Because of its simplicity and mild pH conditions, cyanogen bromide activation is the most common method for preparing affinity gels. Cyanogen bromide is also often used because it reacts with the hydroxyl groups on agarose to form cyanate esters and imidocarbonates. These groups are reacted with primary amines in order to couple the protein onto the agarose matrix, as shown in the figure. Because cyanate esters are more reactive than are cyclic imidocarbonates, the amine will react mostly with the ester, yielding isourea derivatives, and partially with the less reactive imidocarbonate, yielding substituted imidocarbonates.[4]

The disadvantages of this approach include the toxicity of cyanogen bromide and its sensitivity to oxidation. Also, cyanogen bromide activation involves the attachment of a ligand to agarose by an isourea bond, which is positively charged at neutral pH and thus unstable. Consequently, isourea derivatives may act as weak anion exchangers.[4]

Protein cleavage

Cyanogen bromide hydrolyzes peptide bonds at the C-terminus of methionine residues. This reaction is used to reduce the size of polypeptide segments for identification and sequencing.

Mechanism

Cyanogen bromide peptide bond cleavage

The electron density in cyanogen bromide is shifted away from the carbon atom, making it unusually electrophilic, and towards the more electronegative bromine and nitrogen. This leaves the carbon particularly vulnerable to attack by a nucleophile, and the cleavage reaction begins with a nucleophilic acyl substitution reaction in which bromine is ultimately replaced by the sulfur in methionine. This attack is followed by the formation of a five-membered ring as opposed to a six-membered ring, which would entail the formation of a double bond in the ring between nitrogen and carbon. This double bond would result in a rigid ring conformation, thereby destabilizing the molecule. Thus, the five-membered ring is formed so that the double bond is outside the ring, as shown in the figure.

Although the nucleophilic sulfur in methionine is responsible for attacking BrCN, the sulfur in cysteine does not behave similarly. If the sulfur in cysteine attacked cyanogen bromide, the bromide ion would deprotonate the cyanide adduct, leaving the sulfur uncharged and the beta carbon of the cysteine not electrophilic. The strongest electrophile would then be the cyanide nitrogen, which, if attacked by water, would yield cyanic acid and the original cysteine.

Reaction conditions

Cleaving proteins with BrCN requires using a buffer such as 0.1M HCl (hydrochloric acid) or 70% (formic acid).[5] These are the most common buffers for cleavage. An advantage to HCl is that formic acid causes the formation of formyl esters, which complicates protein characterization. However, formic is still often used because it dissolves most proteins. Also, the oxidation of methionine to methionine sulfoxide, which is inert to BrCN attack, occurs more readily in HCl than in formic acid, possibly because formic acid is a reducing acid. Alternative buffers for cleavage include guanidine or urea in HCl because of their ability to unfold proteins, thereby making methionine more accessible to BrCN.[6]

Note that water is required for normal peptide bond cleavage of the iminolactone intermediate. In formic acid, cleavage of Met-Ser and Met-Thr bonds is enhanced with increased water concentration because these conditions favor the addition of water across the imine rather than reaction of the side chain hydroxyl with the imine. Lowered pH tends to increase cleavage rates by inhibiting methionine side chain oxidation.[6]

Side reactions

When methionine is followed by serine or threonine, side reactions can occur that destroy the methionine without peptide bond cleavage. Normally, once the iminolactone is formed (refer to figure), water and acid can react with the imine to cleave the peptide bond, forming a homoserine lactone and new C-terminal peptide. However, if the adjacent amino acid to methionine has a hydroxyl or sulfhydryl group, this group can react with the imine to form a homoserine without peptide bond cleavage.[6] These two cases are shown in the figure.

Organic synthesis

Cyanogen bromide is also widely used in organic synthesis. As stated earlier, the reagent is prone to attack by nucleophiles such as amines and alcohols because of the electrophilic carbon. In the synthesis of cyanamides and dicyanamides, primary and secondary amines react with BrCN to yield mono- and dialkylcyanamides, which can further react with amines and hydroxylamine to yield guanidines and hydroxyguanidines. In the von Braun reaction, tertiary amines react with BrCN to yield disubstituted cyanamides and an alkyl bromide. Cyanogen bromide can be used to prepare aryl nitriles, nitriles, anhydrides, and cyanates. It can also serve as a cleaving agent.[7] Cyanogen bromide can be cyclotrimerized to yield cyanuric bromide:

3 BrCN → (BrCN)3

Toxicity, storage, and deactivation

Cyanogen bromide is moisture-sensitive but can be stored under dry conditions at 2 to 8 °C for extended periods of time.[4]

Cyanogen bromide is volatile, and readily absorbed through the skin or gastrointestinal tract. Therefore, toxic exposure may occur by inhalation, physical contact, or ingestion. It is acutely toxic, causing a variety of nonspecific symptoms. Exposure to even small amounts may cause convulsions or death. LD50 orally in rats is reported as 25–50 mg/kg.[8]

The recommended method to deactivate cyanogen bromide, in a solution not exceeding 60 g/L of BrCN (dilute if necessary), is to add 1 mol/L NaOH and 1 mol/L NaOCl in volumes of ratio 1:1:2 (BrCN solution:NaOH:NaOCl).[9] The aqueous alkali hydroxide instantly hydrolyzes BrCN to alkali cyanide and bromide. The cyanide can then be oxidized by sodium or calcium hypochlorite to the less toxic cyanate ion. Note that deactivation is extremely exothermic and may be explosive.[8]

References

  1. "Cyanogen Bromide - Compound Summary". PubChem Compound. USA: National Center for Biotechnology Information. 26 March 2005. Identification. Retrieved 4 June 2012.
  2. The Merck Index (10th ed.). Rahway, NJ: Merck & Co. 1983. p. 385.
  3. Hermanson, G. T.; Mallia, A. K.; Smith, P. K. (1992). Immobilized Affinity Ligand Techniques. Academic Press. ISBN 978-0123423306.
  4. 4.0 4.1 4.2 "Cyanogen Bromide Activated Matrices" (PDF). Sigma.
  5. Schroeder, W. A.; Shelton, J. B.; Shelton, J. R. (1969). "An Examination of Conditions for the Cleavage of Polypeptide Chains with Cyanogen Bromide". Archives of Biochemistry and Biophysics 130 (1): 551–556. doi:10.1016/0003-9861(69)90069-1.
  6. 6.0 6.1 6.2 Kaiser, R.; Metzka, L. (1999). "Enhancement of Cyanogen Bromide Cleavage Yields for Methionyl-Serine and Methionyl-Threonine Peptide Bonds". Analytical Biochemistry 266 (1): 1–8. doi:10.1006/abio.1998.2945.
  7. Kumar, V. (2005). "Cyanogen Bromide (CNBr)" (PDF). Synlett 2005 (10): 1638–1639. doi:10.1055/s-2005-869872. Art ID: V12705ST.
  8. 8.0 8.1 "Cyanogen Bromide HSDB 708". HSDB. NIH / NLM. 2009-04-07.
  9. Lunn, G.; Sansone, E. B. (1985). "Destruction of Cyanogen Bromide and Inorganic Cyanides". Analytical Biochemistry 147 (1): 245–250. doi:10.1016/0003-2697(85)90034-X. PMID 4025821.

Further reading

External links