N-Acetyl-L-histidine

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N-Acetyl-L-histidine
Category Others
Catalog number BBF-05677
CAS 2497-02-1
Molecular Weight 197.2
Molecular Formula C8H11N3O3

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Specification

Synonyms acetyl-L-histidine; N2-Acetylhistidine; Ac-His-OH
IUPAC Name (2S)-2-acetamido-3-(1H-imidazol-5-yl)propanoic acid
Canonical SMILES CC(=O)NC(CC1=CN=CN1)C(=O)O
InChI InChI=1S/C8H11N3O3/c1-5(12)11-7(8(13)14)2-6-3-9-4-10-6/h3-4,7H,2H2,1H3,(H,9,10)(H,11,12)(H,13,14)/t7-/m0/s1
InChI Key KBOJOGQFRVVWBH-ZETCQYMHSA-N

Reference Reading

1. Ultraviolet spectrophotometric characterization of copper(II) complexes with imidazole N-methyl derivatives of L-histidine in aqueous solution
Enrico Prenesti, Silvia Berto, Pier Giuseppe Daniele Spectrochim Acta A Mol Biomol Spectrosc. 2003 Jan 1;59(1):201-7. doi: 10.1016/s1386-1425(02)00162-2.
In this study we considered pi-methyl-L-histidine (pi-methis) and tau-methyl-L-histidine (tau-methis) as ligands for copper(II) ion, in order to clarify, by means of ultraviolet (UV) spectroscopy in aqueous solution (T = 25 degrees C, I = 0.1 M), some aspects of the co-ordination mode with respect to other ligands of a previous study in which copper(II) complexes of L-histidine, N-acetyl-L-histidine, histamine, L-histidine methyl ester or carnosine were investigated. Particularly, UV spectra (300-400 nm) were recorded on solutions at various pH values, containing each binary system Cu-L; afterwards, an UV absorption spectrum for single complexes was calculated, taking into account the chemical model previously assessed, in order to fulfil a correct spectrum-structure correlation. The problem related to the eventual superimposition of the CT shoulder (approximately 330 nm) to copper(II) of OH- and imidazole pyridine nitrogen groups were now solved by means of a comparison of the UV spectra of dimer species formed by both pi-methis or tau-methis. Finally, copper(II) complex formation with 2,2'-bipyridine was taken into account to compare the behaviour of pyridine (from 2,2'-bipyridine) and pyridine imidazole nitrogens (from pi-methis or tau-methis) with respect to the UV charge transfer process to copper(II) ion.
2. pH responsive histidin-2-ylidene stabilized gold nanoparticles
Adam J Young, Constantin Eisen, Guilherme M D M Rubio, Jia Min Chin, Michael R Reithofer J Inorg Biochem. 2019 Oct;199:110707. doi: 10.1016/j.jinorgbio.2019.110707. Epub 2019 May 10.
N-Heterocyclic carbene-stabilized metal nanoparticles have drawn much attention over the last decade due their strong carbon metal bond. Although several reports show increased stability of such N-heterocyclic carbene-stabilized metal nanoparticles, only limited examples of water-soluble N-heterocyclic carbene stabilized metal nanoparticles are known to date. However, water dispersibility and stability in biologically relevant solvents would be a prerequisite for any biological applications. Drawing from the natural amino acid chiral pool, L-histidine was utilized for preparing chiral NHC ligands in the synthesis of water soluble NHC-stabilized gold nanoparticles. For this purpose, N-acetyl-L-histidine ethyl ester was converted into its imidazolium salt either using methyl iodide or 2-iodopropane as alkylation agent. Subsequent reaction of the imidazolium salt with [Au(SMe2)Cl] yielded the corresponding organometallic gold chloride complex. Histidine-2-ylidene stabilized gold nanoparticles were first generated in organic solvents; the histidine derived capping ligand bore ethyl ester moieties which were saponified, affording water soluble pH-responsive NHC-stabilized gold nanoparticles. These gold nanoparticles show remarkable stability in aqueous solutions, with gold nanoparticle solutions remaining stable after months of storage.
3. N-acetyl-L-histidine, a Prominent Biomolecule in Brain and Eye of Poikilothermic Vertebrates
Morris H Baslow, David N Guilfoyle Biomolecules. 2015 Apr 24;5(2):635-46. doi: 10.3390/biom5020635.
N-acetyl-L-histidine (NAH) is a prominent biomolecule in brain, retina and lens of poikilothermic vertebrates. In fish lens, NAH exhibits an unusual compartmentalized metabolism. It is synthesized from L-histidine (His) and acetyl Co-enzyme A. However, NAH cannot be catabolized by lens cells. For its hydrolysis, NAH is exported to ocular fluid where a specific acylase cleaves His which is then actively taken up by lens and re-synthesized into NAH. This energy-dependent cycling suggested a pump mechanism operating at the lens/ocular fluid interface. Additional studies led to the hypothesis that NAH functioned as a molecular water pump (MWP) to maintain a highly dehydrated lens and avoid cataract formation. In this process, each NAH molecule released to ocular fluid down its gradient carries with it 33 molecules of bound water, effectively transporting the water against a water gradient. In ocular fluid the bound water is released for removal from the eye by the action of NAH acylase. In this paper, we demonstrate for the first time the identification of NAH in fish brain using proton magnetic resonance spectroscopy (MRS) and describe recent evidence supporting the NAH MWP hypothesis. Using MRS, we also document a phylogenetic transition in brain metabolism between poikilothermic and homeothermic vertebrates.

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