Recent advances in exploring the properties and applications of hyaluronan

Hyaluronan(HA)is a naturally occurring polysaccharide in the organism.As one of the main components of the extracellular matrix,it plays an important role in regulating various cellular processes,including proliferation,differentiation,inflammation,and immunity,through interaction with HA receptors.HA is widely found in the human body,particularly in the skin and joints,thus playing a crucial role in the functioning of these tissues.The aging of the skin and the occurrence of osteoarthritis are related to the loss of HA.Supplementing HA in the appropriate areas can delay or prevent these processes.Common methods of HA supplementation include topical application to the skin or injection into the joint cavities,both of which have shown efficacy in restoring HA levels and improving tissue function.In recent years,studies have shown that oral administration of HA can also have similar effects.Oral HA first passes through the gastrointestinal tract and then enters the liver with the blood circulation.Therefore,in addition to supplementing the HA content in the body,oral HA can also exert beneficial effects on the gastrointestinal tract and the liver,such as enhancing the barrier function of the gastrointestinal tract,regulating the intestinal flora,and reducing inflammation.Supplementation of HA has numerous benefits for the skin,orthopedic disorders,gastrointestinal tract and liver.Therefore,it is important to understand the mechanisms through which HA exerts these effects.This article describes the basic properties of HA and reviews its relationship with skin,orthopedic diseases,gastrointestinal tract and liver,as well as its applications in these areas.

Hyaluronan对创面组织中生长因子含量的影响

目的探讨Hyaluronan对创面愈合组织中的生长因子含量的影响。方法将小型猪背部的去中厚皮片创面(共128个)分为实验组和自身对照组,在实验组创面上分别应用0.5%、1.0%及2.0%的Hyaluronan,测定术后第3、7、14、28天各创面愈合组织中的bFGF及EGF含量。结果Hyaluronan能促进创面愈合组织中EGF含量的增加,同时能相对抑制愈合组织中bFGF的增加。结论Hyaluronan通过对创面组织中的生长因子水平的调控,在促进创面愈合的同时能减轻瘢痕的形成。

Golgi localization and dynamics of hyaluronan binding protein 1 (HABP1/p32/C1QBP) during the cell cycle

Hyaluronan binding protein 1 (HABP1) is a negatively charged multifunctional mammalian protein with a unique structural fold. Despite the fact that HABP1 possesses mitochondrial localization signal, it has also been localized to other cellular compartments. Using indirect immunofluorescence, we examined the sub-cellular localization of HABP1 and its dynamics during mitosis. We wanted to determine whether it distributes in any distinctive manner after mitotic nuclear envelope disassembly or is dispersed randomly throughout the cell. Our results reveal the golgi localization of HABP1 and demonstrate its complete dispersion throughout the cell during mitosis. This distinctive distribution pattern of HABP1 during mitosis resembles its ligand hyaluronan, suggesting that in concert with each other the two molecules play critical roles in this dynamic process.

Determination of Hyaluronan by Spectroscopic Methods

Hyaluronan is a kind of polysaccharide with high molecule weight, hs structure is relatively complicated and tertiary structure exists among the HA molecules when reaching to o certain solution concentration . FT- IR spectrum has been acquired to shou the groups and their ascription in HA. The results of FT-IR spectrum in this essay accords well with that issued by ASTM. As to the newly appearing absorption peaks, sensible explanation has been given, In ADDITION , Ramon spectrum has been employed as a proof for the result of the FT-IR spectnun. Based on the preliminary acknowledge of the functional groups in HA, circular dichroism of the material has also been explored.

Biology of hyaluronan: Insights from genetic disorders of hyaluronan metabolism

Hyaluronan is a rapidly turned over component of the vertebrate extracellular matrix. Its levels are determined, in part, by the hyaluronan synthases, HAS1, HAS2, and HAS3, and three hyaluronidases, HYAL1, HYAL2 and HYAL3. Hyaluronan binding proteins also regulate hyaluronan levels although their involvement is less well understood. To date, two genetic disorders of hyaluronan metabolism have been reported in humans: HYAL1 deficiency(Mucopolysaccharidosis IX) in four individuals with joint pathology as the predominant phenotypic finding and HAS2 deficiency in a single person having cardiac pathology. However, inherited disorders and induced mutations affecting hyaluronan metabolism have been characterized in other species. Overproduction of hyaluronan by HAS2 results in skin folding and thickening in shar-pei dogs and the naked mole rat, whereas a complete deficiency of HAS2 causes embryonic lethality in mice due to cardiac defects. Deficiencies of murine HAS1 and HAS3 result in a predisposition to seizures. Like humans, mice with HYAL1 deficiency exhibit joint pathology. Mice lacking HYAL2 have variably penetrant developmental defects, including skeletal and cardiac anomalies. Thus, based on mutant animal models, a partial deficiency of HAS2 or HYAL2 might be compatible with survival in humans, while complete deficiencies of HAS1, HAS3, and HYAL3 may yet be recognized.

Structural and functional evidence for two separate oligosaccharide binding sites of Pasteurella multocida hyaluronan synthase

Pasteurella multocida hyaluronan synthase (PmHAS) is a bi-functional glycosyltransferase, containing a β1,3-glucuronyltransferase and β1,4-N-acetylglucosaminetransferase domain. PmHAS catalyzes the elongation of hyaluronan (HA) through the sequential addition of single monosaccharides to the non-reducing end of the hyaluronan chain. Research is focused on the relation between the length of the HA oligosaccharide and the single-step elongation kinetics from HA4 up to HA9. It was found that the turnover number kcat increased with length to maximum values of 11 and 14 s-1 for NAc- and UA-transfer, respectively. Interestingly, the specificity constant kcat/KM increased with polymer length from HA5 to HA7 to a value of 44 mM-1s-1, indicating an oligosaccharide binding site with increasing specificity towards a heptasaccharide at the UA domain. The value of kcat/KM remained moderately constant around 8 mM-1s-1 for HA4, HA6, and HA8, indicating a binding site with significantly lower binding specificity at the NAc domain than at the UA domain. These findings are further corroborated by a structural homology model of PmHAS, revealing two distinct sites for binding of oligosaccharides of different sizes, one in each transferase domain. Structural alignment studies between PmHAS and glycosyltransferases of the GT-A fold showed significant similarity in the binding of the UDP-sugars and the orientation of the acceptor substrate. These similarities in substrate orientation in the active site and in essential amino acid residues involved in substrate binding were utilized to localize the two HA oligosaccharide binding sites.

Biological Evaluation of Tissue-Engineered Cartilage Using Thermoresponsive Poly(<i>N</i>-isopropylacrylamide)-Grafted Hyaluronan

In order to contribute to the development of minimally invasive surgery techniques for autologous chondrocyte implantation, a novel self-assembling biomaterial consisting of thermoresponsive poly(N-isopropylacrylamide)-grafted hyaluronan (PNIPAAm-g-HA) has been synthesized as an injectable scaffold for cartilage tissue engineering. The aim of this study was to investigate the efficacy and cytocompatibility of PNIPAAm-g-HA to normal chondrocytes by using reverse transcription-polymerase chain reaction (RT-PCR) analysis and histochemical staining in preliminary in vitro and in vitro experiments. Hematoxylin and eosin staining showed homogeneous distribution of cells in the PNIPAAm-g-HA hydrogel in 3-dimensional in vitro cultivation. Alcian blue staining also indicated that abundant extracellular matrix formation, including acidic glycosaminoglycans, occurred in tissue-engineered cartilage over time in vitro. Cartilage-related gene expression patterns, which were tested in rabbit normal chondrocytes embedded in the hydrogel, were almost maintained for 4 weeks. Transforming growth factor-β1 (TGF-β1) stimulation enhanced the expression of SRY-related HMG box-containing gene 9 (Sox9) and type X collagen genes suggesting promotion of chondrogenic differentiation. Histochemical evaluation showed neocartilage formation following subcutaneous implantation of the chondrocyte-gel mixture in nude mice. Furthermore, TGF-β1 stimulation promoted production and maturation of the extracellular matrix of the in situ tissue engineered hyaline cartilage. These data suggested that PNIPAAm-g-HA could be a promising biomaterial, i.e., a self-assembling and injectable scaffold for cartilage tissue engineering.

Injectable <i>in situ</i>crosslinkable hyaluronan-polyvinyl phosphonic acid hydrogels for bone engineering

A novel injectable hydrogel that was synthesized by in situ crosslinking of hyaluronan and polyvinyl phosphonic acid was proposed in this study. Fourier transform infrared spectrum (FT-IR) analysis, scanning electron microscope (SEM), pH measurement, and biodegradation test were used to confirm its characteristics. The results permitted to prove successful crosslinking, observe the inner morphology of hydrogel and pore sizes distribution, and determine the decomposition of hydrogel components during incubation time. Result of pH measurement showed that the pH scale of hydrogel decreased when volume of PVPA increased. As a consequence, it affected the cytotoxicity value, cell proliferation, and cell growth behaviors of each hydrogel. Optical microscope observation showed that chondroblasts cell proliferated well on HA-PVPA hydrogel. Therefore, these results suggest that the new injectable hydrogel is appropriate for bone/cartilage regeneration applications.

Bacteriostatic Effects of Hyaluronan-Based Bioresorbable Membrane

Purpose: The purpose of this study is to determine the presence of bacteriostatic effects of hyaluronan-based bioresorbable membrane (HA/CMC) on selected major bacterial strains in digestive organs. Methods: We firstly evaluated the growth inhibition effect of HA/CMC for E. coli and S. aureus by determining the optical density (OD)650 in the incubation medium. At second, to determine the viable counts of bacteria, total adenosine triphosphate (ATP) were measured with five groups;several concentrations of HA/CMC and control. Results: OD curve gradually elevated and reached to plateau at 4 hours in E. coli. and 6 hours in S. aureus. After reaching plateau, the growth inhibition of both strains was statistically significantly correlated to the concentrations of HA/CMC. The ATP productions had statistically significant differences at 6 hours after incubation and inhibited in dose-dependence of a well-dissolved HA/CMC. Conclusion: HA/CMC may have dose-dependently bacteriostatic effects on S. aureus and E. coli.

Effects of hyaluronan oligosaccharides on apoptosis ofhuman gingival fibroblasts

An?increased?content?of?low?molecular?weight (LMW)- HA?was?found?in?human?gingiva?during?the?initial phase of?periodontitis. A?number?of?functions?have?been?described?for LMW-HA?in?inflammatory?processes.?It?is?also?demonstrated?that?LMWHA?induces?apoptosis?in?chondrocytes?and?tumor?cells,?however, effects of?LMWHA on the apoptosis?of?gingival?fibroblasts?(GFs) remain?unclear. The?purpose?of?this?study?was?to?investigate?the effects?of HA?oligosaccharides?(HAoligo) on?the apoptosis of GFs. GFs were?isolated?from?palatal?gingival?tissues around?the upper?first?premolars of eight youth?(6 -10?years?old)?and eight adult?(26 -35?years?old) subjects.?Cultured?GFs?were?subjected?to?the?analyses,?ELISA?for?cell?proliferation,?quantitative real?time-PCR?for?gene?expression?of?Bcl-2,?and?caspase-3?assay?for?apoptotic potency. Proliferative?activity?of?cultured?GFs was increased?

Study on Chemical Cross-linking Modification of Hyaluronan and the Biocompatibility of its Derivatives

Objective: Prepare cross-linked HA gels with higher mechanical stability, lower degradation velocity and desirable biocompatibility,so as to extend the usage of HA.Method:1.Test molecular weight of HA (Mr_ HA ) by viscosimetry;2.prepare cross-linked HA gels by DVS, GTA, DEC;3.discuss the cross-linking and degradation procedure;4.evaluate the biocompatibility of the best HA gels. Results:The mechanical stability and durability to degradation of HA-DVS gels are superior to those of other gels, and when HA:DVS = 40:1(g/g), at 35℃ and in 0.2 M NaOH solution, the HA-DVS gel shows the best mechanical stability, and its cytotoxicity reaches class I, hemolysis ratio is lower than 5%. Conclusion:Our HA-DVS gel can be used to prepare biologic scaffolds.

Study on Preparation and Release of Dexamethasone Hyaluronan Microspheres

Hyaluronan (HA), the consistent glycosaminoglycans in extracellular matrix, is a kind of biomaterials with wonderful biocompatibility. To develop drug release system (DDS) with HA as drug carrier is a new hotspot in the field of pharmaceutics. In this paper, we applied technique of ultrosound and reversed phase (Water/Oil) emulsification to develop dexamethasone (DEX)-HA-STMP cross-linking microspheres (DEX-HA MS) with STMP as cross-linker. DEX-HA MS has a wonderful shape and property of dispersion. There is a negative correlation between diameter of DEX-HA MS and the content of cross-linker, or the content of emulsifier, and a positive correlation between the diameter and CHA . When CHA≤1%,DEX/HA≤1/10 (g/g),there is a positive correlation between the factors mentioned below and drug loading (DL%)/loading efficiency (LE%),the content of STMP, the content of emulsifier,CHA and the content of DEX. DEX-HA-MS can realize function of slow release. In vitro drug release experiment shows that cumulative release (CR%) of DEX-HA MS fits in with pervasion-corrosion equation, and there is a negative correlation between the content of STMP, CHA and CR%, a positive correlation between emulsifier and CR%. When DEX/HA≤1/5 (g/g) there is a negative correlation between the content of DEX and CR%.

内源性透明质酸对小鼠牙乳头细胞增殖的影响

目的:探究内源性透明质酸(hyaluronan, HA)对小鼠牙乳头细胞(mouse dental papilla cells, mDPCs)增殖的影响。方法:对出生后2.5 d的小鼠腹腔注射5-乙炔基-2′脱氧尿嘧啶核苷(5-ethynyl-2′-deoxyuridine, EdU)标记快速增殖细胞;体外分离培养mDPCs,使用不同浓度透明质酸酶(hyaluronidase, HAase)降解HA,细胞计数试剂盒(cell counting kit-8,CCK-8)法及EdU法检测细胞增殖;使用流式细胞术检测细胞周期分布和凋亡;转染siHyal2抑制HA降解,EdU法检测细胞增殖。结果:HA主要表达在小鼠切牙根尖慢增殖间充质细胞周围,而在转运扩增细胞(transit-amplifying cells, TACs)表达下降;CCK-8结果显示,相比对照组,800μg/mL HAase明显促进细胞增殖(P<0.0001);EdU检测及流式细胞术结果显示,HAase处理48 h后,细胞DNA合成增加,S期细胞比率明显增加(P<0.01),并抑制早期细胞凋亡(P<0.05);与之相反,当HA积聚在mDPCs细胞周,细胞增殖受到抑制(P<0.01)。结论:内源性HA与mDPCs增殖密切相关,HA分解可促进细胞增殖;而局部HA的积聚则抑制细胞增殖。

血清1-磷酸鞘氨醇联合透明质酸检测对结直肠癌的诊断及预后价值

目的:观察分析结直肠癌(CRC)患者血清1-磷酸鞘氨醇(S1P)和透明质酸(HA)的水平变化及相关性,探讨其对结直肠癌诊断和预后评估的临床价值。方法:收集47例结直肠癌患者(结直肠癌组)、30例肠道良性疾病患者(良性疾病组)和38名健康的体检者(健康对照组)的临床资料,并检测所有受试者的血清S1P和HA水平。利用Spearman相关性分析评估两者相关性。采用受试者工作特征(ROC)曲线评估S1P、HA、癌胚抗原(CEA)和糖类抗原19-9(CA19-9)单独和联合诊断CRC的效能。结果:血清S1P水平在健康对照组、良性疾病组及结直肠癌组中逐次升高(P<0.05)。结直肠癌组血清HA水平高于健康对照组(P<0.05),然而良性疾病组的血清HA水平与结直肠癌组和健康对照组之间的差异无统计学意义(P>0.05)。根据Spearman相关性分析结果,结直肠癌组血清S1P水平和HA水平之间存在正相关关系(r=0.406,P<0.05)。ROC曲线结果显示,S1P、HA、CEA、CA19-9单独和联合诊断CRC的曲线下面积分别为0.871、0.642、0.694、0.593及0.916。术后CRC患者血清HA水平显著降低(P<0.001),但术后血清S1P水平与术前差异无统计学意义(P>0.05)。结论:血清S1P与HA结合检测在结直肠癌的辅助诊断及预后评估中具有一定的临床价值。

FOXM1靶向HMMR对骨肉瘤细胞凋亡和自噬影响

目的探讨叉头盒M1(FOXM1)转录因子通过靶向透明质酸介导的运动受体(HMMR)对骨肉瘤(OS)细胞凋亡和自噬的影响。方法使用慢病毒载体构建敲低FOXM1和过表达HMMR的OS细胞系,将转染空载慢病毒的细胞作为对照组,转染sh-FOXM1慢病毒的细胞作为敲低FOXM1组,转染sh-FOXM1慢病毒和OE-HMMR慢病毒的细胞作为过表达HMMR组。采用Western blot方法检测正常成骨细胞(hFOB1.19)和OS细胞(U-2OS)中FOXM1蛋白的表达;通过流式细胞术检测对照组、敲低FOXM1组和过表达HMMR组U-2OS细胞的凋亡率;采用Western blot方法检测对照组和敲低FOXM1组OS细胞中HMMR蛋白、自噬蛋白(LC3Ⅰ/Ⅱ)、凋亡相关蛋白(Cleaved-Caspase3、Bax)的表达以及过表达HMMR组OS细胞中自噬蛋白(LC3Ⅰ/Ⅱ)的表达。结果FOXM1在U-2OS细胞中的表达明显高于hFOB1.19细胞(t=38.780,P<0.005)。与对照组相比,敲低FOXM1组U-2OS细胞凋亡率显著增加(t=3.517,P<0.05),Cleaved-Caspase3、Bax、LC3Ⅰ/Ⅱ和HMMR蛋白表达显著下降(t=3.155~6.334,P<0.05),而过表达HMMR恢复了敲低FOXM1导致的凋亡率增加和自噬抑制(F=31.00、160.20,P<0.05)。结论FOXM1敲低通过降低HMMR蛋白的表达促进OS细胞凋亡和抑制OS细胞自噬。

Targeting hyaluronan for the treatment of pancreatic ductal adenocarcinoma

Progression of cancer is often associated with interactions between cancer cells and extracellular matrix(ECM) surrounding them. Increasing evidence has suggested that accumulation of hyaluronan(HA), a major component of ECM, provides a favorable microenvironment for cancer progression. Pancreatic ductal adenocarcinoma(PDAC) is characterized typically by a dense desmoplastic stroma with a large amount of HA, making this molecule as an attractive target for therapy. Several studies have shown efficacy of inhibitors of HA synthesis or signaling for the treatment of PDAC. Recent studies have also demonstrated substantial improvements in the effects of chemotherapy by a targeted depletion of stromal HA in PDAC using an enzymatic agent. Thus, targeting HA has been recognized as a promising therapeutic strategy to treat this highly aggressive neoplasm. In this review article, we summarize our current understanding of the role of HA in the progression of PDAC and discuss possible therapeutic approaches targeting HA.

透明质酸在肿瘤细胞可塑性调控中作用的研究进展

透明质酸(hyaluronan,HA)是细胞外基质的重要成分,在肿瘤间质中异常潴留,参与肿瘤微环境的重构。据报道,HA及其相关代谢酶、受体与肿瘤细胞可塑性改变密切相关,在肿瘤干细胞干性维持、上皮-间充质转换(epithelial to mesenchymal transition,EMT)、获得性耐药等过程中均发挥重要的调节作用。本文对HA在调节肿瘤细胞可塑性中作用的研究进展进行了综述。

Collagen/hyaluronan based hydrogels releasing sulfated hyaluronan improve dermal wound healing in diabetic mice via reducing inflammatory macrophage activity

Sustained inflammation associated with dysregulated macrophage activation prevents tissue formation and healing of chronic wounds.Control of inflammation and immune cell functions thus represents a promising approach in the development of advanced therapeutic strategies.Here we describe immunomodulatory hyaluronan/collagen(HA-AC/coll)-based hydrogels containing high-sulfated hyaluronan(sHA)as immunoregulatory component for the modulation of inflammatory macrophage activities in disturbed wound healing.Solute sHA downregulates inflammatory activities of bone marrow-derived and tissue-resident macrophages in vitro.This further affects macrophage-mediated pro-inflammatory activation of skin cells as shown in skin ex-vivo cultures.In a mouse model of acute skin inflammation,intradermal injection of sHA downregulates the inflammatory processes in the skin.This is associated with the promotion of an anti-inflammatory gene signature in skin macrophages indicating a shift of their activation profile.For in vivo translation,we designed HA-AC/coll hydrogels allowing delivery of sHA into wounds over a period of at least one week.Their immunoregulatory capacity was analyzed in a translational experimental approach in skin wounds of diabetic db/db mice,an established model for disturbed wound healing.The sHA-releasing hydrogels improved defective tissue repair with reduced inflammation,augmented pro-regenerative macrophage activation,increased vascularization,and accelerated new tissue formation and wound closure.

Th1 cytokines promote T-cell binding to antigen-presenting cells via enhanced hyaluronan production and accumulation at the immune synapse

Hyaluronan(HA)production by dendritic cells(DCs)is known to promote antigen presentation and to augment T-cell activation and proliferation.We hypothesized that pericellular HA can function as intercellular‘glue’directly mediating T cell–DC binding.Using primary human cells,we observed HA-dependent binding between T cells and DCs,which was abrogated upon pre-treatment of the DCs with 4-methylumbelliferone(4-MU),an agent which blocks HA synthesis.Furthermore,T cells regulate HA production by DCs via T cell-derived cytokines in a T helper(Th)subset-specific manner,as demonstrated by the observation that cell-culture supernatants from Th1 but not Th2 clones promote HA production.Similar effects were seen upon the addition of exogenous Th1 cytokines,IL-2,interferon c(IFN-c)and tumor necrosis factor a(TNF-a).The critical factors which determined the extent of DC–T cell binding in this system were the nature of the pre-treatment the DCs received and their capacity to synthesize HA,as T-cell clones which were pre-treated with monensin,added to block cytokine secretion,bound equivalently irrespective of their Th subset.These data support the existence of a feedforward loop wherein T-cell cytokines influence DC production of HA,which in turn affects the extent of DC–T cell binding.We also document the presence of focal deposits of HA at the immune synapse between T-cells and APC and on dendritic processes thought to be important in antigen presentation.These data point to a pivotal role for HA in DC–T cell interactions at the IS.