Structural studies of the capsular polysaccharides from Klebsiella types 8 and 82, a reinvestigation

The structures of the capsular polysaccharides elaborated by Klebsiella types 8 (K8) and 82 (K82) have been reinvestigated. N.m.r. spectroscopy of the original and chemically modified polysaccharides was the principal method used. It is concluded that the polysaccharides are composed of repeating units having the following structures. (Formula: see text). The presence of L-glutamic acid, linked as an amide to the carboxyl group of a uronic acid, has not been observed hitherto in bacterial polysaccharides.     

Affinity adsorbents consisting of nucleic acids immobilized via bisoxirane activated polysaccharides.

An easy and efficient procedure for the immobilization of polynucleotide ligands to bisoxirane activated insoluble polysaccharides has been elaborated and is described in this paper. The resulting materials have been applied to the chromatography of DNA polymerase I, and RNA polymerase from E.coli. Because of their extraordinary stability to temperature, formamide, and alkaline conditions they seem to be particularly useful adsorbents for nucleic acid hybridization.     

Rapid estimation of polysaccharide content in complex microbial culture media

A rapid gravimetric assay for estimation of polysaccharide content in complex culture media was developed and validated. The quantitative assay showed great selectivity for the determination of xylan and pectin, eliminating all interferences from other medium components. In addition, our data showed this protocol could also be applied to the estimation of other polysaccharides in liquid media such as cellulose Avicel^®, chitin, starch and crude hemicellulose. Therefore, this method represents a useful tool for monitoring the in vitro microbial degradation of polysaccharides.     

A dye binding assay for the quantification of soluble and cell-bound acidic polysaccharides produced by red algae

Polysaccharides produced in technical scale from red algae serve in a variety of industrial applications. Ruthenium red (RR) is a cytochemical stain which has been used to visualize these mostly acidic polysaccharides in light microscopy. The binding of RR to algal polysaccharides is highly dependent on the ionic strength of the surrounding medium. The dye is firmly bound at low ionic strength, but is released at increasing salt concentrations. These properties were exploited to develop a new method to quantify the amount of cell wall material synthesized by algal cells under different physiological conditions. Soluble or extracted polysaccharides are quantified by a dot-blot procedure with subsequent image analysis, while cell-bound polysaccharides are determined in situ by a dye-binding assay followed by photometry. In comparison to the current methods of quantification, the new assay is quick, reliable, and avoids extensive use of hazardous chemicals.     

A sensitive staining method for detecting acidic polysaccharides in cellulose acetate and agarose gels

A sensitive staining method has been developed for the detection of acidic polysaccharides in cellulose acetate and agarose gels. The method is based on the precipitation of bovine serum albumin by acidic polysaccharides at acidic pH values and the subsequent staining of precipitated protein with amido black or Coomassie brilliant blue R-250 stains. The detection limit of acidic polysaccharides is 15-40 ng on cellulose acetate strips and 50-150 ng on agarose plates. The sensitivity of the described staining technique is of the same order for a wide range of acidic polysaccharides of different origin in contrast to Alcian blue and toluidine blue stains, which detect only mucopolysaccharides of animal origin at comparable levels. The method was also applied to the colorimetric quantitative determination of acidic polysaccharides after electrophoretic separation.     

Studies of molecular-weight distribution for hydrolysis products from some Klebsiella capsular polysaccharides

Gel-permeation chromatography has been used to determine the molecular-weight distribution of the products at various stages of acid hydrolysis of some capsular polysaccharides from klebsiella bacteria. Structurally significant oligosaccharides, which are believed to correspond closely to the chemical repeating units in the polysaccharide molecules, were detected together with products having higher molecular weights, which are clearly aggregates of these oligosaccharides. This constitutes good supporting evidence for the view that relatively simple sequences of sugars are repeated throughout the entire molecular structure of these polysaccharides, and quantitative information for the polysaccharides from three different Klebsiella strains (serotyped as k54, K4, and K64, respectively) has been obtained by this procedure. The study of the polysaccharide from Klebsiella K-type 54 has afforded both independent corroboration and some extension of available data.     

Intra and inter generic homology in polysaccharide structure ofRhizobium andAlcaligenes

A study was conducted on the structure of extracellular, water-soluble polysaccharides from 5 different strains ofRhizobium viz. R. trifolii J60 andR. meliloti strains J7017, 202, 204 and 207. All these polysaccharides were found to contain glucose and galactose in the approximate molar ratio of 7:1. Methylation analysis revealed these polysaccharides to contain (1 → 3), (1 → 6), (1 → 4), (1 → 4, 1 → 6)-linked D-glucose residues, (1 → 3)-linked D-galactose and nonreducing terminal D-glucose attached to pyruvate. These polysaccharides were also found to be acylated by both acetyl and succinyl residue. This structure was found to be similar to that of succinoglycan, a succinic acid-containing water-soluble, extra-cellular polysaccharide elaborated byAlcaligenes faecalis var.myxogenes 10C3. This similarity in structure of polysaccharides from two different species ofRhizobium and also the polysaccharide produced byAlcaligenes has been discussed.     

An HPLC method for the determination of acetyl and pyruvyl groups in polysaccharides

A method for the quantitative analysis of pyruvate and acetate groups in polysaccharides has been developed, using HPLC on a cation exchange resin in the protonated form and u.v. detection at 210 nm. Procedures for release of acetate and pyruvate from polysaccharides are described.In the case of xanthan gum, most of the pyruvate is removed if the sample is autoclaved in water during preparation, and about 25% is lost if autoclaved in 0·1 m sodium chloride solution.     

食药用真菌多糖抗氧化作用研究进展

食药用真菌多糖由于其独特的生理活性,目前正成为国内外众多学科领域研究的热点之一。综述了食药用真菌多糖抗氧化作用研究现状、作用机理及其构效与量效关系,并对其发展前景进行了展望,旨在为其深入研究和开发利用提供参考。     

Studies on the blood-anticoagulant activity of sulphated polysaccharides with different uronic acid content

The anticoagulant activities of sulphated alginic acids, amylose, cellulose, chitosan, curdlan, dextran, guaran, laminaran and locust bean gum have been studied. The alginic acids have been partially reduced and some of the neutral polysaccharides have been partially oxidised at C-6 of the glycopyranosyl residues. The activities of sulphated polymers containing different proportions of uronic acid and neutral sugar residues have been compared.The results suggest that polysaccharides with an average of at least one sulphate group on each monomeric unit, a molecular weight higher than 10 000 and a high proportion of sulphated primary hydroxyl functions will display activity in the activated, partial thromboplastin time assay (APTT). Sulphated guaran and locust bean gum had the highest activities of the polymers investigated (70 IU/mg, heparin has 130-50 IU/mg). In the concentration range investigated, none of the sulphated polymers showed any significant activity in an anti-factor X_a assay.     

ALCIAN BLUE: A QUANTITATIVE AQUEOUS ASSAY FOR ALGAL ACID AND SULFATED POLYSACCHARIDES1

Alcian Blue, a cationic copper phthalocyanine dye, complexes with the anionic carboxyl and half-ester sulfate groups of acidic algal polysaccharide in aqueous solution to form an insoluble precipitate. The quantity of dye removed from solution is proportional to the quantity of polyanion in solution, and this principle forms the basis for the quantitative determination of acid and/or sulfated algal polysaccharides. The assay is linear between 0 and 100 μg/ml agar, alginic acid, carrageenan, pectin and Porphyridium aerugineum Geit. polysaccharide. In addition, the technique is used to determine the anion density of acid polysaccharides on a molar or weight equivalency basis.     

An ultraviolet-spectrophotometric method with 2-cyanoacetamide for the determination of the enzymatic degradation of reducing polysaccharides.

A rapid, facile, and sensitive uv-spectrophotometric assay has been developed for the determination of the enzymatic degradation of polysaccharides that generates reducing sugars. The assay was carried out with 2-cyanoacetamide in a single test tube. The solution was left at pH 9 by the addition of borate buffer within 5 min. Measurement of the reaction mixture at 274 nm allows a simple determination up to 600 mumol/liter of reducing sugars. The coefficient of variation was less than 2% on all measurements. The assay was developed with pectin and polygalacturonic acid from apples and has been compared with the Somogyi-Nelson method. The new assay was then exemplarily used for the determination of the enzymatic hydrolysis products of pectin from cotton.     

Anti-bacterial,anti-scavenging and cytotoxic activity of garden cress polysaccharides

Plants polysaccharides are an infinite stock of drug composites with varying pharmacological and biological activities. The present investigation aimed to examine the antibacterial, anti-scavenging and cytotoxic potential of garden cress (GC) polysaccharides. The antibacterial effects vs Escherichia coli and as well as Staphylococcus aureus of GC polysaccharides were examined by means of agar diffusion assay, minimum inhibitory concentration (MIC), outer and inner cell membrane permeability. Antioxidant potential of the GC polysaccharides were performed by free radical DPPH scavenging, superoxide anion scavenging, hydroxyl radical scavenging, reducing power potential assay, and hydrogen peroxide method. Cytotoxicity potential of GC polysaccharides were evaluated by MTT assay in human cervical (HeLa) and liver carcinoma (HepG2) cell lines. The findings showed that GC polysaccharides MIC were 1.06 and 0.56 mg mL⁻¹ against E. coli and S. aureus, respectively. Compared to the standard inhibitor, the GC polysaccharides showed essential inhibitor assays in a very dose dependent approach, and notable actions to scavenge reactive oxygen species (ROS) are also due to the large quantities of hydrophilic polyphenols. The IC₅₀ values of all tested parameters were measured against standard ascorbic acid antioxidant agent. The GC polysaccharides diminish the cell viability percentage of HeLa and HepG2 in a concentration dependent manner. GC polysaccharides at a dose of 500 µg ml⁻¹ exhibited higher anti-tumor activity in both HeLa (65.33 ± 3.75%) and HepG2 (60.33 ± 3.48%). The findings obtained in this study indicate that GC polysaccharides has antibacterial and has a possible source of natural antioxidant and also has cytotoxic effect on different carcinoma cell lines.     

Investigating the candidacy of the serotype specific rhamnan polysaccharide based glycoconjugates to prevent disease caused by the dental pathogen <Emphasis Type="Italic">Streptococcus mutans</Emphasis>

Dental caries remains a major health issue and the Gram-positive bacterium Streptococcus mutans is considered as the major pathogen causing caries. More recently, S. mutans has been recognised as a cause of endocarditis, ulcerative colitis and fatty acid liver disease along with the likelihood of increased cerebral hemorrhage following a stroke if S. mutans is present systemically. We initiated this study to examine the vaccine candidacy of the serotype specific polysaccharides elaborated by S. mutans. We have confirmed the carbohydrate structures for the serotype specific rhamnan containing polysaccharides from serotypes c, f and k. We have prepared glycoconjugate vaccines using the rhamnan containing polymers from serotypes f and k and immunised mice and rabbits. We consistently obtained a robust immune response to the glycoconjugates with cross-reactivity consistent with the structural similarities of the polymers from the different serotypes. We developed an opsonophagocytic assay which illustrated the ability of the post-immune sera to facilitate opsonophagocytic killing of the homologous and heterologous serotypes at titers consistent with the structural homologies. We conclude that glycoconjugates of the rhamnan polymers of S. mutans are a potential vaccine candidate to target dental caries and other sequelae following the escape of S. mutans from the oral cavity.     

A method of intravital study of pulmonary microcirculation in closed-chest cats

The methods of intravital study of the cat lungs have been updated. A device has been designed for the investigation of microvessels in extended lung areas of spontaneously breathing closed-chest cats. The principles for quantitative analysis of microcirculatory lung parameters have been elaborated. These new methods allow the study of important natural phenomena of the lung microvascular functions.     

Development and validation of an NMR-based identity assay for bacterial polysaccharides

A method utilizing NMR spectroscopy has been developed to confirm the identity of bacterial polysaccharides used to formulate a polyvalent pneumococcal polysaccharide vaccine. The method is based on 600 MHz proton NMR spectra of individual serotype-specific polysaccharides. A portion of the anomeric region of each spectrum (5.89 to 4.64 ppm) is compared to spectra generated for designated reference samples for each polysaccharide of interest. The selected region offers a spectral window that is unique to a given polysaccharide and is sensitive to any structural alteration of the repeating units. The similarity of any two spectral profiles is evaluated using a correlation coefficient (rho), where rho >/= 0.95 between a sample and reference profile indicates a positive identification of the sample polysaccharide. This method has been shown to be extremely selective in its ability to discriminate between serotype-specific polysaccharides, some of which differ by no more than a single glycosidic linkage. Furthermore, the method is rapid and does not require extensive sample manipulations or pretreatments. The method was validated as a qualitative identity assay and will be incorporated into routine quality control testing of polysaccharide powders to be used in preparation of the polyvalent pneumococcal vaccine PNEUMOVAX 23. The specificity and reproducibility of the NMR-based identity assay is superior to the currently used colorimetric assays and can be readily adapted for use with other bacterial polysaccharide preparations as well.     

A simple method for hyaluronic acid quantification in culture broth

The carbazole assay has been used for determination of the percentage of hyaluronic acid in biological fluids. However, it is difficult to measure the concentration of hyaluronic acid in culture broth because glucose and polysaccharides remaining after cultures can react with sulfuric acid and carbazole. The glucose and polysaccharide remnants must be completely removed in order to get the correct value for hyaluronic acid. The turbidity assay, another method for estimating the concentration of hyaluronic acid, is based on the formation of insoluble complexes between hyaluronic acid and cetyltrimethylammonium bromide. This method is very easy and fast compared with the carbazole assay. Because concentrations of hyaluronic acid measured by the turbidity assay were ranged around 100% of those measured by the carbazole assay, the content of hyaluronic acid in culture broth can be determined by the turbidity assay. The turbidity method also has the advantage of being safer than the carbazole assay.     

近红外光谱测定灵芝子实体多糖含量

灵芝具有多种药理活性,多糖是其主要活性成分之一.目前灵芝多糖的定量常采用的比色法,使用比较繁琐,也缺乏一定的安全环保性.应用近红外光谱对灵芝进行多糖定量分析,发现对子实体直接分析存在定量不准的问题.为了快速准确地评估灵芝子实体多糖含量,本研究采用对灵芝子实体水提物进行近红外光谱检测与分析,由此建立了较好的定量模型.该模...     

Profiling Carbohydrate-Receptor Interaction with Recombinant Innate Immunity Receptor-Fc Fusion Proteins

The recognition of bacteria, viruses, fungi, and other microbes is controlled by host immune cells, which are equipped with many innate immunity receptors, such as Toll-like receptors, C-type lectin receptors, and immunoglobulin-like receptors. Our studies indicate that the immune modulating properties of many herbal drugs, for instance, the medicinal fungus Reishi (Ganoderma lucidum) and Cordyceps sinensis, could be attributed to their polysaccharide components. These polysaccharides specifically interact with and activate surface receptors involved in innate immunity. However, due to the complexity of polysaccharides and their various sources from medicinal fungi, quantitative analysis of medicinal polysaccharide extracts with regard to their functions represents a major challenge. To profile carbohydrate-immune receptor interactions, the extracellular domains of 17 receptors were cloned as Fc-fusion proteins, such that their interactions with immobilized polysaccharides could be probed in an enzyme-linked immunosorbent assay. The results show that several innate immune receptors, including Dectin-1, DC-SIGN, Langerin, Kupffer cell receptor, macrophage mannose receptor, TLR2, and TLR4, interact with the polysaccharide extracts from G. lucidum (GLPS). This analysis revealed distinct polysaccharide profiles from different sources of medicinal fungi, and the innate immune receptor-based enzyme-linked immunosorbent assay described here can serve as a high-throughput profiling method for the characterization and quality control of medicinal polysaccharides. It also provides a means to dissect the molecular mechanism of medicinal polysaccharide-induced immunomodulation events.