658-69-5

Basic information

• Product Name: L-PHENYLALANINE-UL-14C
• Synonyms: PHENYLALANINE, L-, [14C(U)];L-PHENYLALANINE [U-14 C];L-PHENYLALANINE-UL-14C;(S)-(-)-phenylalanine-UL-14C;L-Phenylalanine-UL-14C hydrochloride
• CAS NO: 658-69-5
• Molecular Formula: C9H11NO2
• Molecular Weight: 183.35
• Mol File: 658-69-5.mol
• Article Data: 685

Chemical Properties

• Appearance: /
• Storage Temp.: 2-8°C
• CAS DataBase Reference: L-PHENYLALANINE-UL-14C(CAS DataBase Reference)
• NIST Chemistry Reference: L-PHENYLALANINE-UL-14C(658-69-5)
• EPA Substance Registry System: L-PHENYLALANINE-UL-14C(658-69-5)

Safety Data

• Hazard Codes: Xi
• Statements: 36/37/38
• Safety Statements: 26-36
• RIDADR: UN 2910 7
• Hazardous Substances Data: 658-69-5(Hazardous Substances Data)

Usage

General Description

L-PHENYLALANINE-UL-14C is a radiolabeled form of the amino acid phenylalanine. It contains a carbon-14 isotope, making it useful for tracking and studying the metabolism and uptake of phenylalanine in various biological systems. Phenylalanine is an essential amino acid that plays a crucial role in protein synthesis and serves as a precursor for the neurotransmitters dopamine, norepinephrine, and epinephrine. By using L-PHENYLALANINE-UL-14C, researchers can gain insights into the metabolic pathways and functions of phenylalanine in living organisms, including humans. This radiolabeled compound is widely used in biochemical and pharmacological research, as well as in medical imaging and diagnostic procedures.

Upstream product

• 1155-48-2 2-benzoylaminocinnamic acid 
• 7647-01-0 hydrogenchloride 
• 127478-97-1 (5-benzyl-3,6-dioxo-piperazin-2-yliden)-acetic acid methyl ester 
• 92965-71-4 5-benzyl-2-phenyl-imidazolidin-4-one 
• 156-06-9 2-oxo-3-(phenyl)propionic acid 
• 7732-18-5 water 
• 2835-06-5 phenylglycin 
• 110-89-4 piperidine 
• 4289-95-6 N-formyl-phenylalanine 
• 13505-32-3 N-tosyl-(S)-phenylalanine 
• 2577-90-4 methyl (2S)-2-amino-3-phenylpropanoate 
• 2901-75-9 (R,S)-N-acetyl phenylalanine 
• 42291-22-5 N-acetyl dehydrophenylalanyl-(S)-phenylalanine 
• 15080-84-9 Phe-Met 

Downstream Products

• 109717-32-0 N-hexahydroazepin-2-ylidene-DL-phenylalanine 
• 197392-59-9 N-(quinoline-2-carbonyl)-DL-phenylalanine 
• 37534-65-9 D-2-carbamoylamino-3-phenylpropionic acid 
• 1170-07-6 N-(N,N-phthaloyl-glycyl)-L-phenylalanine 
• 90235-83-9 2-amino-5-benzyl-1,5-dihydro-imidazol-4-one 
• 105909-73-7 2,5-Dimethyl-4-(phenylmethyl)oxazole 
• 63531-84-0 4-sulfo-phenylalanine 
• 350-09-4 N-trifluoroacetyl-L-phenylalanine 
• 7153-00-6 N-[(Ξ)-2-(2,4-dichloro-phenoxy)-propionyl]-L-phenylalanine 
• 32945-04-3 N-carboxymethyl-L-phenylalanine 
• 6710-91-4 bis-N,N-carboxymethyl-(S)-phenylalanine 
• 102026-88-0 N-(5-acetylamino-2,4-dinitro-phenyl)-L-phenylalanine 
• 101269-34-5 N-(2,2-bis-acetylamino-propionyl)-L-phenylalanine 
• 56145-93-8 salicyloyl-phenylalanine 

Relevant articles and documents

Enhanced carboxypeptidase efficacies and differentiation of peptide epimers

Carboxypeptidases enzymatically cleave the peptide bond of C-terminal amino acids. In humans, it is involved in enzymatic synthesis and maturation of proteins and peptides. Carboxypeptidases A and Y have difficulty hydrolyzing the peptide bond of dipeptides and some other amino acid sequences. Early investigations into different N-blocking groups concluded that larger moieties increased substrate susceptibility to peptide bond hydrolysis with carboxypeptidases. This study conclusively demonstrates that 6-aminoquinoline-N-hydroxysuccimidyl carbamate (AQC) as an N-blocking group greatly enhances substrate hydrolysis with carboxypeptidase. AQC addition to the N-terminus of amino acids and peptides also improves chromatographic peak shapes and sensitivities via mass spectrometry detection. These enzymes have been used for amino acid sequence determination prior to the advent of modern proteomics. However, most modern proteomic methods assume that all peptides are comprised of L-amino acids and therefore cannot distinguish L-from D-amino acids within the peptide sequence. The majority of existing methods that allow for chiral differentiation either require synthetic standards or incur racemization in the process. This study highlights the resistance of D-amino acids within peptides to enzymatic hydrolysis by Carboxypeptidase Y. This stereoselectivity may be advantageous when screening for low abundance peptide stereoisomers.

Highly Stable Zr(IV)-Based Metal-Organic Frameworks for Chiral Separation in Reversed-Phase Liquid Chromatography

Separation of racemic mixtures is of great importance and interest in chemistry and pharmacology. Porous materials including metal-organic frameworks (MOFs) have been widely explored as chiral stationary phases (CSPs) in chiral resolution. However, it remains a challenge to develop new CSPs for reversed-phase high-performance liquid chromatography (RP-HPLC), which is the most popular chromatographic mode and accounts for over 90% of all separations. Here we demonstrated for the first time that highly stable Zr-based MOFs can be efficient CSPs for RP-HPLC. By elaborately designing and synthesizing three tetracarboxylate ligands of enantiopure 1,1′-biphenyl-20-crown-6, we prepared three chiral porous Zr(IV)-MOFs with the framework formula [Zr6O4(OH)8(H2O)4(L)2]. They share the same flu topological structure but channels of different sizes and display excellent tolerance to water, acid, and base. Chiral crown ether moieties are periodically aligned within the framework channels, allowing for stereoselective recognition of guest molecules via supramolecular interactions. Under acidic aqueous eluent conditions, the Zr-MOF-packed HPLC columns provide high resolution, selectivity, and durability for the separation of a variety of model racemates, including unprotected and protected amino acids and N-containing drugs, which are comparable to or even superior to several commercial chiral columns for HPLC separation. DFT calculations suggest that the Zr-MOF provides a confined microenvironment for chiral crown ethers that dictates the separation selectivity.

Reconstruction of Hyper-Thermostable Ancestral L-Amino Acid Oxidase to Perform Deracemization to D-Amino Acids

L-amino acid oxidases (LAAOs) with broad substrate specificity can be used in the deracemization of D,L-amino acids (D,L-AAs) to their D-enantiomers. Hyper-thermostable LAAO (HTAncLAAO) was designed through a combination of manual sequence data mining and ancestral sequence reconstruction. Soluble expression of HTAncLAAO (>50 mg/L) can be achieved using an E. coli system. HTAncLAAO, which recognizes seven L-AAs as substrates, exhibits extremely high thermal stability and long-term stability; the t1/2 value was 95 °C and 99 % ee, D-enantiomer). These results suggest that HTAncLAAO is an excellent biocatalyst to perform this deracemization.