Dextran partial

Leuconostoc mesenteroides strain SF-4 dextran partially hydrolyzed by acid. 

Leuconostoc mesenteroides NRRL B-1375 (Birmingham) dextran partially hydrolyzed by add. 

Acrylamide graft copolymers such as those with starch (qv)(131), dextran (132), and lignin (qv) (133), have been studied to try to reduce copolymer costs. A general disadvantage of acrylamide copolymers is greater cost compared to partially hydroly2ed polyacrylamides. 

The basis for the separation is that when two polymers, or a polymer and certain salts, are mixed together in water, they are incompatible, leading to the formation of two immiscible but predominantly aqueous phases, each rich in only one of the two components [Albertsson, op. cit. Kula, in Cooney and Humphrey (eds.), op. cit., pp. 451 71]. A phase diagram for a polyethylene glycol (PEG)-Dextran, two-phase system is shown in Fig. 22-85. Proteins are known to distribute unevenly between these phases. This uneven distribution can be used for the selective concentration and partial purification of the products. Partitioning between the two phases is controlled by the polymer molecular weight and concentration, protein net charge and... 

In addition to polymer standards, a number of broad distribution, water-soluble polymers can be characterized on TSK-PW columns using universal calibration. These include both fully and partially hydrolyzed PVA, PAAM, PEE, and dextran. PVA, the world s largest-volume, synthetic, water-soluble polymer, was first successfully separated on TSK-PW columns by Hashimota et al. (10). In the 1980s, the use of low-angle, laser light-scattering detection... 

FU(1), chitosan-5FU(2), a-l,4-polygalactosamine-5FU(3), partially N-acetylated a-l,4-polygalactosamine-5FU(4), hyaluronic acid-5FU(5), dextran-5FU(6), and 6-0-carboxymethyl chitin(CM-chitin)-5FU(7). 

The presence of three hydroxyl groups per glucose unit was shown by the preparation of a triacetate and a tribenzoate. Six or seven methyla-tions (using dimethyl sulfate and concentrated alkali) of dextran did not raise the methoxyl content above 41% (theoretical maximum 45.6%). Also, Purdie methylations (using methyl iodide and silver oxide) and methylation with thallium ethoxide and methyl iodide were ineffective in raising the methoxyl content of methylated dextran above 43.5%. The maximum theoretical methoxyl content was eventually attained by modified Muskat methylations. 6 Partially methylated dextran suspended in anisole solution was treated with sodium in liquid ammonia, and the sodium salt of methylated dextran thus formed was allowed to react with methyl iodide. The methoxyl content of the partially methylated dextran was raised by three such methylations from 42% to 45.5% and by five such methylations from 30% to 45.4%. 

Claims have recently been made61 that the dextran of L. mesenteroides may serve as an efficient substitute for blood plasma. Solutions of partially-hydrolyzed dextran in saline gave favorable results when injected intravenously into experimental animals. Preliminary clinical tests were promising. 

For maximum efficiency, methylation should be a single-phase reaction and so those methods employing aqueous alkali are most suitable for water-soluble compounds and the Purdie method for non-polar compounds. A carbohydrate which is initially soluble in water e.g., starch, dextran) may be less soluble when partially methylated and for this reason an inert solvent e.g., acetone, dioxane, carbon tetrachloride) is often introduced during the later stages of a methylation with dimethyl sulfate. It is interesting to note that methyl a-D-glucopyranoside forms a trithallium derivative which is insoluble in water and consequently the introduction of more than three methoxyl groups by the Menzies method... 

The chemical structures of five dextrans were partially determined by methylation, and found to be branched molecules having the following types of substitution (a) 6-0 and 3,6-di-O, (b) 6-0, 3-0, and 3,6-di-O, (c) 6-0,3,6-di-O, and 2,3-di-O, (d) 6-0, 4-0, and 3,4-di-O, and (e) 6-0 and 2,3-di-O. At 27° and pH 7 (external, Me4Si standard), the 13C shifts ofO-substituted, non-anomeric carbon atoms were C-2 (76.5), C-3 (81.6), and C-4 (79.5). The C-l resonances were also recorded, and may be used for reference purposes. Some variation of chemical shifts, relative to each other, was observed with changing temperature. (The work serves to emphasize the importance of accurately measuring the temperature of the solution when determining chemical shifts.102)... 

A lipophilic gel, namely, Sephadex LH-20, has found application in studies of partially acetylated dextrans. In describing a modified procedure for the replacement of the O-acetyl groups in such dextrans by O-methyl groups prior to acid hydrolysis and identification of the fragments (which indicates the distribution of the substituents in... 

It was reported by Jourdain et al. (2008) that it was impossible to make a proper emulsion with sodium caseinate alone at pH = 4 because of the very low protein solubility close to pI. Nevertheless, a fine stable emulsion (c/43 1.0 pm) could easily be prepared when dextran sulfate was present in a modest amount. In contrast, the monodisperse bilayer emulsion could not be prepared at low pH because the primary caseinate-stabilized emulsion was already either partially aggregated (pH = 2) or completely insoluble (pH = 4) under these conditions. 

This degradation has also been applied151 to the dextran produced by Leuconostoc mesenteroides NRRL B-512, which is composed of (1 — 6)-linked a-D-glycopyranose residues, about 5% of which carry a side chain linked to 0-3 (partial structure 87). Tritylation of... 

Method A. The rationale of method A is that HDL and LDL are separated by selective precipitation of LDL by dextran sulfate and Mg2+ after the reaction between LDL and reconstituted HDL containing radiolabeled CE by CETP. The method was originally described by Kato et al. [77], The assay mixtures consist of reconstituted [14C]CE-HDL as the donor for CE, LDL as the acceptor, 5,5 -dithiobis-2-nitrobenzoic acid, bovine serum albumin (BSA), partially purified CETP, and a test sample in Eppendorf tubes (1.5 ml). After a 30-min incubation at 37°C, the reaction is terminated by the addition of an LDL-precipitation solution. After standing for 20 min in an ice bath, the assay mixtures are centrifuged, and the supernatant solution containing [14C]CE-HDL is analyzed for radioactivity. Furthermore, the [14C]CE-LDL precipitate is also analyzed for radioactivity if necessary. Usually the blank and control transfer values are about 6% and 34% of initial [14C]CE-HDL added under the assay conditions, respectively. 

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