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Histidine mixtures

Potentiometric determination of the pH of L-histidine solutions with and without D-glucose at 40° showed that, at initial pH values between 5 and 6.5, the pH remained constant for both samples. When the initial pH was above 6.5, alkali had to be added to the D-glucose-histidine mixture in order to maintain the pH.137 Chromatographic evidence shows that other basic amino acids (such as lysine and arginine) also react238 with D-glucose... [Pg.111]

Crystallization Method. Such methods as mechanical separation, preferential crystallisation, and substitution crystallisation procedures are included in this category. The preferential crystallisation method is the most popular. The general procedure is to inoculate a saturated solution of the racemic mixture with a seed of the desired enantiomer. Resolutions by this method have been reported for histidine (43), glutamic acid (44), DOPA (45), threonine (46), A/-acetyl phenylalanine (47), and others. In the case of glutamic acid, the method had been used for industrial manufacture (48). [Pg.278]

Describe the expected elution pattern for a mixture of aspartate, histidine, isoleucine, valine, and arginine on a column of Dowex-50. [Pg.106]

Capillary tube isotachophoresis using a potential gradient detector is another technique that has been applied to the analysis of alcohol sulfates, such as sodium and lithium alcohol sulfates [303]. The leading electrolyte solution is a mixture of methyl cyanate and aqueous histidine buffer containing calcium chloride. The terminating electrolyte solution is an aqueous solution of sodium octanoate. [Pg.285]

Hiroshima, 721 histidine, 443, 774 hole, 195 homeostasis, 386 HOMO, 126, 580 homogeneous alloy, 202 homogeneous catalyst, 565 homogeneous equilibria, 362 homogeneous mixture, F53 homolytic dissociation, 80 homonuclear diatomic molecule, 103 Hooke s law, 92 hormone, 670 horsepower, A4, 791 hour, A4 HPLC, 354 HRF products, 723 HTSC, 192 Humphreys series, 51 Hund, F 35 Hund s rule, 35, 37 Hurricane Rita, 144 hyaluronic acid, 344 hybrid orbital, 109 hybridization bond angle, 131 molecular shape, 111 hydrangea color, 463 hydrate, F32 hydrate isomer, 676 hydration, 178 hydrazine, 627... [Pg.1033]

L-Histidine (50 mg) was placed in the flask. The flask was again flushed with nitrogen. Tetrahydrofuran (30 mL) was added and the mixture was stirred. [Pg.170]

The enantiomeric purity of protected amino acids used in peptide synthesis can be determined by pre-column partial deprotection followed by derivatization with Marfey s reagent (116). The Marfey diastereoisomers can be easily resolved and determined by RP-HPLC using an ODS-Hypersil column288. Fifteen amino acids collected from mammalian tissues were derivatized with Marfey s reagent and subjected to two-dimensional TLC. Each individual spot (enantiomeric mixture of a diasteroisomer) was then resolved by RP-HPLC. Except for tyrosine (46) and histidine (117), subnanomole quantities of enantiomers could be analyzed289,290. [Pg.1089]

Affinity chromatography and related techniques (e.g., thiol chromatography and IMAC) are widely used for preparative isolation because they enable a single protein or class of proteins to be selectively purified from very complex mixtures. They may be occasionally used as analytical tools. For example, protein A affinity chromatography has been used for quantitative analysis of immunoglobulins in ascites fluid.45 Information about surface-accessible histidine and phosphate groups may be obtained using IMAC. [Pg.60]

Racemic mixtures of underivatized amino acids Cu (II)-N - -decyl-L-histidine on ODS silica Water-Cu(II) acetate -1- organic modifier (85/15) 228... [Pg.471]

Briefly, liposomes (10mM) were incubated for 30minutes at 37°C for egg phosphatidylcholine (EPC) and at 60°C for HSPC-based liposomes with 50 X 10 dpm of methylamine (1 x 10 dpm/mole). At the end of incubation an aliquot of this mixture was passed down a Sephadex G-50 minispin column equilibrated in 10 mM histidine-sucrose buffer 10%, pH 6.7 buffer. Liposomes were eluted at the column void volume and separated from the unencapsulated methylamine. The concentration of liposomes in the original liposomal dispersion and in the void volume fraction was determined from the organic phosphorus (phospholipid) concentration (see section Lipid Quantification and Chemical Stability above) (10,49,53). [Pg.20]

The proximal calcium binding site is coupled to the heme group by virtue of the fact that one of its ligands, Thrl71, is adjacent to the proximal histidine residue, Hisl70 (Fig. 4). The results of site-directed mutagenesis studies at this position are awaited with interest. An illustration of the importance of both calcium sites to the structure and function of HRP C is afforded by the need to incorporate calcium as a component of in vitro folding mixtures to obtain active recombinant enzyme from solubilized inclusion bodies (64). [Pg.135]

MCD spectroscopy in range 300 to 2000 nm at both ambient and liquid helium (4.2 K) temperatures can yield information about the spin, oxidation, and coordination states of each heme in a multiheme protein such as CCP (75). This technique, in combination with low-temperature X-band EPR spectroscopy, was used to great effect in characterizing the properties of the fully oxidized and MV forms of the P. aeruginosa CCP in solution. At 4.2 K, both hemes in the oxidized enzyme are low-spin ferric, with diagnostic features in the near infrared-MCD (NIR-MCD) spectrum consistent with one heme with His/Met axial coordination and the other with bis-histidine axial coordination this is entirely consistent with the crystal structure. In contrast, at room temperature only the low-potential (bis-histidine coordinated) heme in the C-terminal domain remains completely low-spin, whereas the high-potential (His/Met coordinated) heme exists as mixture of high- and low-spin forms 58). [Pg.191]

Rainbow trout, Salmo gairdneri, are primarily visual feeders, but also use their chemical senses for foraging. They prefer a diet flavored with squid extract to non-treated food. A synthetic mixture of 18 amino acids, two amines, and lactic acid was very active. Only L-forms triggered responses D-forms were even repellent. Only two combinations of amino acids were active tyrosine, phenylalanine, and lysine and tyrosine phenylalanine, and histidine (Adron and Mackie, 1978). [Pg.340]

Three primary tests are incorporated in the health effects area. The microbial mutagenesis assay is based on the property of selected Salmonella typhimurium mutants to revert from a histidine requiring state to prototrophy due to exposre to various classes of mutagens. The test can detect nanogram quantities of mutagens and has been adapted to mimic some mammalian metabolic processes by the addition of a mammalian liver microsomal fraction. The test is used as a primary screen to determine the mutagenic activity of complex mixtures or component fractions. [Pg.40]

A base-catalyzed Pictet-Spengler reaction of (S)-histidine with benzaldehyde was recently reported to yield a mixture of diastereomers, 59 % trans and 22 % cis 139). [Pg.200]


See other pages where Histidine mixtures is mentioned: [Pg.379]    [Pg.263]    [Pg.379]    [Pg.263]    [Pg.146]    [Pg.511]    [Pg.518]    [Pg.53]    [Pg.2]    [Pg.14]    [Pg.252]    [Pg.4]    [Pg.463]    [Pg.403]    [Pg.17]    [Pg.1193]    [Pg.1221]    [Pg.379]    [Pg.76]    [Pg.143]    [Pg.356]    [Pg.193]    [Pg.304]    [Pg.238]    [Pg.136]    [Pg.42]    [Pg.72]    [Pg.24]    [Pg.79]    [Pg.361]    [Pg.55]    [Pg.968]    [Pg.973]    [Pg.323]    [Pg.638]    [Pg.475]    [Pg.188]    [Pg.968]   
See also in sourсe #XX -- [ Pg.83 , Pg.87 , Pg.89 ]




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