glycans

聚糖
  • 文章类型: Journal Article
    目的:用异双官能低分子量聚乙二醇(PEG)(600和1395Da)修饰聚烯丙胺盐酸盐(PAH),以及随后的甘露糖附着,葡萄糖,或乳糖糖PEG,可导致形成具有凝集素结合亲和力和窄尺寸分布的聚胺磷酸盐纳米颗粒(PANs)。
    方法:尺寸,多分散性,用透射电子显微镜(TEM)对糖基化聚乙二醇化PAN的内部结构进行了表征,动态光散射(DLS)和小角度X射线散射(SAXS)。荧光相关光谱(FCS)用于研究标记的乙二醇-聚乙二醇化PAN的缔合。形成纳米颗粒的聚合物链的数量由纳米颗粒形成后聚合物的互相关函数的幅度变化来确定。SAXS和荧光交叉相关光谱用于研究PAN与凝集素的相互作用:伴刀豆球蛋白A与甘露糖修饰的PAN,和Jacalin用乳糖改性的。
    结果:Glyco-PEG化PAN是高度单分散的,具有几十纳米的直径和低电荷,和对应于具有高斯链的球体的结构。FCS显示PAN是单链纳米颗粒或由两个聚合物链形成。伴刀豆球蛋白A和Jamalin对糖聚乙二醇化的PAN显示出特异性相互作用,其亲和力高于牛血清白蛋白。
    OBJECTIVE: Modification of polyallylamine hydrochloride (PAH) with heterobifunctional low molecular weight polyethylene glycol (PEG) (600 and 1395 Da), and subsequent attachment of mannose, glucose, or lactose sugars to PEG, can lead to formation of polyamine phosphate nanoparticles (PANs) with lectin binding affinity and narrow size distribution.
    METHODS: Size, polydispersity, and internal structure of glycosylated PEGylated PANs were characterized by transmission electron microscopy (TEM), dynamic light scattering (DLS) and small angle X-ray scattering (SAXS). Fluorescence correlation spectroscopy (FCS) was used to study the association of labelled glycol-PEGylated PANs. The number of polymer chains forming the nanoparticles was determined from the changes in amplitude of the cross-correlation function of the polymers after formation of the nanoparticles. SAXS and fluorescence cross-correlation spectroscopy were used to investigate the interaction of PANs with lectins: concanavalin A with mannose modified PANs, and jacalin with lactose modified ones.
    RESULTS: Glyco-PEGylated PANs are highly monodispersed, with diameters of a few tens of nanometers and low charge, and a structure corresponding to spheres with Gaussian chains. FCS shows that the PANs are single chain nanoparticles or formed by two polymer chains. Concanavalin A and jacalin show specific interactions for the glyco-PEGylated PANs with higher affinity than bovine serum albumin.
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  • 文章类型: Journal Article
    分子动力学(MD)是一种用于计算原子和分子运动的方法,广泛应用于科学的多个方面。它涉及计算模拟,这使得它,乍一看,不容易接近。几种进行分子模拟的自动化工具的兴起使研究人员能够浏览MD的各个步骤。这使得能够阐明蛋白质的结构特性,否则无法分析,如糖基化的影响。糖基化决定了调节其溶解度的蛋白质的物理化学和生物学特性,稳定性,对蛋白水解的抗性,互动伙伴,酶活性,绑定和识别。鉴于聚糖链的高构象和组成多样性,使用常规分析技术评估它们对蛋白质结构的影响是具有挑战性的。在这份手稿中,我们提出了一个循序渐进的工作流程,以构建和执行针对SARS-CoV-2的SPIKE糖蛋白的糖蛋白MD分析,以评估聚糖在结构稳定和抗体闭塞中的影响.
    Molecular Dynamics (MD) is a method used to calculate the movement of atoms and molecules broadly applied to several aspects of science. It involves computational simulation, which makes it, at first glance, not easily accessible. The rise of several automated tools to perform molecular simulations has allowed researchers to navigate through the various steps of MD. This enables to elucidate structural properties of proteins that could not be analyzed otherwise, such as the impact of glycosylation. Glycosylation dictates the physicochemical and biological properties of a protein modulating its solubility, stability, resistance to proteolysis, interaction partners, enzymatic activity, binding and recognition. Given the high conformational and compositional diversity of the glycan chains, assessing their influence on the protein structure is challenging using conventional analytical techniques. In this manuscript, we present a step-by-step workflow to build and perform MD analysis of glycoproteins focusing on the SPIKE glycoprotein of SARS-CoV-2 to appraise the impact of glycans in structure stabilization and antibody occlusion.
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  • 文章类型: Clinical Trial
    慢性移植物抗宿主病(cGvHD)是一种全身性同种免疫和自身免疫性疾病,是异基因造血干细胞移植(alloHSCT)的主要晚期并发症。该疾病的特征在于体液免疫应答的稳态改变。免疫球蛋白G(IgG)糖蛋白是体液免疫应答的主要效应分子。IgG糖基化的变化与许多自身免疫性疾病有关。在美国国立卫生研究院(NIH)的213名cGvHD患者的队列中通过液相色谱法进行IgG糖基化分析。结果显示,关于cGvHDNIH关节/筋膜和皮肤评分,疾病活动和全身免疫抑制的强度。ROC分析证实,使用实验室参数和与cGvHD相关的炎症标志物(嗜酸性粒细胞计数,补体成分C3和C4以及炎症标志物:白蛋白,CRP和血小板计数)。这项研究表明,IgG糖基化可能在cGvHD病理中起重要作用。进一步的研究可能有助于对疾病生物学的理解,并导致临床生物标志物的开发,以允许个性化的方法来治疗慢性GvHD。
    Chronic graft-versus-host disease (cGvHD) is a systemic alloimmune and autoimmune disorder and a major late complication of allogeneic hematopoietic stem cell transplantation (alloHSCT). The disease is characterized by an altered homeostasis of the humoral immune response. Immunoglobulin G (IgG) glycoprotein is the main effector molecule of the humoral immune response. Changes in IgG glycosylation are associated with a number of autoimmune diseases. IgG glycosylation analysis was done by the means of liquid chromatography in the National Institutes of Health (NIH) cohort of 213 cGvHD patients. The results showed statistically significant differences with regards to cGvHD NIH joint/fascia and skin score, disease activity and intensity of systemic immunosuppression. ROC analysis confirmed that IgG glycosylation increases specificity and sensitivity of models using laboratory parameters and markers of inflammation associated with cGvHD (eosinophil count, complement components C3 and C4 and inflammation markers: albumin, CRP and thrombocyte count). This research shows that IgG glycosylation may play a significant role in cGvHD pathology. Further research could contribute to the understanding of the disease biology and lead to the clinical biomarker development to allow personalized approaches to chronic GvHD therapy.
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  • 文章类型: Journal Article
    背景:低子宫内膜容受性是影响辅助生殖技术(ART)成功植入的主要因素之一。子宫内膜薄型不孕患者的累积临床妊娠率明显低于子宫内膜正常患者。薄子宫内膜低接受性的分子病理生理学仍未得到充分研究。我们已经研究了不育妇女的薄子宫内膜中管腔和腺上皮细胞顶表面的糖萼的组成。
    方法:本研究纳入了32例接受体外受精(IVF)的输卵管腹膜不孕症患者。在自然月经周期中获得子宫内膜样品。患者分为两组:子宫内膜正常(≥8mm)和子宫内膜薄(<8mm)。使用六种生物素化的凝集素(UEA-I,MAL-II,SNA,VVL,ECL,ConA)和抗LeY和MECA-79单克隆抗体(MAb)。
    结果:考虑到聚糖结合单克隆抗体的调节特异性的复合聚糖分析显示,与正常子宫内膜相比,薄子宫内膜的管腔上皮细胞顶表面上MECA-79聚糖的表达减少了1.3倍;这种缺乏可能对植入产生不利影响,因为MECA-79聚糖是L-选择素的配体并介导细胞间相互作用。含有2型单位Galβ1-4GlcNAcβ(LacNAc)但在GlcNAcβ的6-OH上缺乏磺基残基的聚糖,并与MECA-79MAb结合;它们可以被认为是子宫内膜容受性的潜在标志物。凝集素染色的聚糖在腔和腺上皮细胞的顶表面上的表达没有显着差异。在子宫内膜薄型和复发性种植失败的患者中,发现二岩藻糖基化寡糖LeY在腔和腺上皮细胞顶表面的表达之间存在相关性。对于富含甘露糖的聚糖显示了类似的关系。
    结论:薄型子宫内膜上皮区室中关键聚糖表达的特定特征可能对子宫内膜功能层的形态发生至关重要,并解释了其低接受性。
    BACKGROUND: Low endometrial receptivity is one of the major factors affecting successful implantation in assisted reproductive technologies (ART). Infertile patients with thin endometrium have a significantly lower cumulative clinical pregnancy rate than patients with normal endometrium. Molecular pathophysiology of low receptivity of thin endometrium remains understudied. We have investigated composition of glycocalyx of the apical surface of luminal and glandular epithelial cells in thin endometrium of infertile women.
    METHODS: Thirty-two patients with tubal-peritoneal infertility undergoing in vitro fertilization (IVF) were included in the study. Endometrial samples were obtained in a natural menstrual cycle. Patients were divided into two groups: patients with normal endometrium (≥8 mm) and with thin endometrium (< 8 mm). Histochemical and immunohistochemical analysis of paraffin-embedded endometrial samples was performed using six biotinylated lectins (UEA-I, MAL-II, SNA, VVL, ECL, Con A) and anti-LeY and MECA-79 monoclonal antibodies (MAbs).
    RESULTS: Complex glycans analysis taking into account the adjusted specificity of glycan-binding MAbs revealed 1.3 times less expression of MECA-79 glycans on the apical surface of the luminal epithelial cells of thin endometrium compared to normal endometrium; this deficiency may adversely affect implantation, since MECA-79 glycans are a ligand of L-selectin and mediate intercellular interactions. The glycans containing a type-2 unit Galβ1-4GlcNAcβ (LacNAc) but lacking sulfo-residues at 6-OH of GlcNAcβ, and binding to MECA-79 MAbs were found; they can be considered as potential markers of endometrium receptivity. Expression of the lectins-stained glycans on the apical surfaces of the luminal and glandular epithelial cells did not differ significantly. Correlation between the expression of difucosylated oligosaccharide LeY on the apical surfaces of the luminal and glandular epithelial cells was found in patients with thin endometrium and recurrent implantation failure. A similar relationship was shown for mannose-rich glycans.
    CONCLUSIONS: Specific features of key glycans expression in epithelial compartments of thin endometrium may be essential for morphogenesis of the endometrial functional layer and explain its low receptivity.
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  • 文章类型: Journal Article
    成年雌性红颈鸵鸟(Struthiocameluscamelus)的生殖道糖基化,当意外地将头部撞死时,在子宫中携带完全形成的钙化卵时,使用凝集素组织化学对漏斗样本进行了检查,大号,子宫和阴道.在某些情况下,在神经氨酸酶预处理后,用23种凝集素染色后,描述了腔上皮和下面腺体中的聚糖。纤毛和非纤毛细胞在腔上皮的所有水平都很明显,后者充满了丰富的糖基化分泌颗粒。纤毛细胞也表现出糖基化,在大号,这些细胞通常比非纤毛细胞染色更强烈。高甘露糖和复杂的N-聚糖,α1,6-连接的岩藻糖基和唾液酸残基存在于整个管道中,并且完全不存在GalNAcα1,3(LFuca1,2)Galβ1,3/4GlcNAc1-和稀有末端GalNAcα1-残基。α1,2-连接的岩藻糖作为H2抗原和Ley在腔上皮中也很少见,在腺体中完全不存在。除漏斗外,末端半乳糖存在于管腔上皮中。腺体上皮表现出与腔上皮相似的糖基化,除了在大细胞中存在显着差异,并且在这里腺体充满了大的分泌颗粒,不像其余的腺体.管道的每个部分都有自己特定的糖基化模式,这可能与卵的形成阶段有关。
    Glycosylation of the reproductive tract of an adult female red-necked ostrich (Struthio camelus camelus) carrying a fully formed calcified egg in her uterus when accidently killed by a blow to the head was examined using lectin histochemistry on samples from the infundibulum, magnum, uterus and vagina. Glycans in the luminal epithelium and underlying glands were described after staining with 23 lectins after neuraminidase pre-treatment in some cases. Ciliated and non-ciliated cells were evident at all levels in the luminal epithelium, the latter full of richly glycosylated secretory granules. The ciliated cells also showed glycosylation and, in the magnum, these cells often stained more intensely than the non-ciliated cells. High mannose and complex N-glycans, α1,6-linked fucosyl and sialic acid residues were present throughout the tract and there was a complete absence of GalNAcα1,3(LFucα1,2)Galß1,3/4GlcNAcß1- and rare terminal GalNAcα1- residues. Fucose in α1,2-linkage as H2 antigen and Ley was also rare in the luminal epithelium and completely absent in glands. Terminal galactose was present in the luminal epithelium apart from in the infundibulum. Gland epithelium showed similar glycosylation to the luminal epithelium except in the magnum where there were significant differences and here the glands were packed full of large secretory granules, unlike the glands in the rest of the tract. Each section of the tract had its own specific pattern of glycosylation which could be related to the stage of egg formation.
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  • 文章类型: Journal Article
    肺癌是美国女性癌症死亡的主要原因,占女性癌症死亡人数的比例与乳腺癌大致相同,子房,和子宫癌合并。靶向血浆糖组学代表了肺癌非侵入性诊断和预后生物标志物的有希望的来源。这里,通过自下而上的聚糖“节点”分析方法分析了参加女性流行病学肺癌(WELCA)研究的208例肺癌患者和207例年龄匹配的对照。Glycan特征,量化为单个分析信号,包括2个连接的甘露糖,α2-6唾液酸化,β1-4分支,β1-6分支,4-链接的GlcNAc,和触角岩藻糖基化,在所有阶段均表现出区分病例与对照组的能力(ROCAUC:0.68-0.92)并预测患者的生存率(风险比:1.99-2.75)。在I-II阶段观察到显著的聚糖特征改变。诊断和预后的聚糖特征大多独立于吸烟状况,年龄,性别,和肺癌的组织学亚型。
    Lung cancer is the leading cause of cancer death in women living in the United States, which accounts for approximately the same percentage of cancer deaths in women as breast, ovary, and uterine cancers combined. Targeted blood plasma glycomics represents a promising source of noninvasive diagnostic and prognostic biomarkers for lung cancer. Here, 208 samples from lung cancer patients and 207 age-matched controls enrolled in the Women Epidemiology Lung Cancer (WELCA) study were analyzed by a bottom-up glycan \"node\" analysis approach. Glycan features, quantified as single analytical signals, including 2-linked mannose, α2-6 sialylation, β1-4 branching, β1-6 branching, 4-linked GlcNAc, and antennary fucosylation, exhibited abilities to distinguish cases from controls (ROC AUCs: 0.68-0.92) and predict survival in patients (hazard ratios: 1.99-2.75) at all stages. Notable alterations of glycan features were observed in stages I-II. Diagnostic and prognostic glycan features were mostly independent of smoking status, age, gender, and histological subtypes of lung cancer.
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  • 文章类型: Journal Article
    我们提供了有关男性泌尿生殖道血吸虫病(UGS)的诊断方法的更新,并强调UGS令人满意的尿液抗原诊断远远落后于肠道血吸虫病。在应用基于尿液的现场护理试条测定的情况下,循环阴极抗原(CCA)测试,现在提倡。特别提到男性生殖器血吸虫病(MGS),我们更加重视寄生虫学检测方法和超声检查对内生殖器的临床评估.与在定义女性生殖器血吸虫病临床标准方案方面取得的进展不同,MGS定义不充分。虽然尿液过滤和显微镜检查血吸虫卵是MGS的一种方便但容易出错的替代方法,我们描述了一种新的低成本采样和直接可视化方法,用于精液中卵子的计数。使用来自马拉维湖沿岸渔民的纵向队列研究中MGS的示例性临床病例,对诊断需求的组合进行评估,包括:使用症状学问卷,尿液分析(鸡蛋计数和CCA测量),精液分析(卵子计数,循环阳极抗原测量和实时聚合酶链反应分析)以及便携式超声检查的临床评估。
    We provide an update on diagnostic methods for the detection of urogenital schistosomiasis (UGS) in men and highlight that satisfactory urine-antigen diagnostics for UGS lag much behind that for intestinal schistosomiasis, where application of a urine-based point-of-care strip assay, the circulating cathodic antigen (CCA) test, is now advocated. Making specific reference to male genital schistosomiasis (MGS), we place greater emphasis on parasitological detection methods and clinical assessment of internal genitalia with ultrasonography. Unlike the advances made in defining a clinical standard protocol for female genital schistosomiasis, MGS remains inadequately defined. Whilst urine filtration with microscopic examination for ova of Schistosoma haematobium is a convenient but error-prone proxy of MGS, we describe a novel low-cost sampling and direct visualization method for the enumeration of ova in semen. Using exemplar clinical cases of MGS from our longitudinal cohort study among fishermen along the shoreline of Lake Malawi, the portfolio of diagnostic needs is appraised including: the use of symptomatology questionnaires, urine analysis (egg count and CCA measurement), semen analysis (egg count, circulating anodic antigen measurement and real-time polymerase chain reaction analysis) alongside clinical assessment with portable ultrasonography.
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  • 文章类型: Journal Article
    The synthesis of oligosaccharides and other carbohydrate derivatives is of relevance for the advancement of glycosciences both at the fundamental and applied level. For many years, glycosyl hydrolases (GHs) have been explored to catalyze the synthesis of glycosidic bonds. In particular, retaining GHs can catalyze a transglycosylation (T) reaction that competes with hydrolysis (H). This has been done either employing controlled conditions in wild type GHs or by engineering new mutants. The goal, which is to increase the T/H ratio, has been achieved with moderate success in several cases despite the fact that the molecular basis for T/H modulation are unclear. Here we have used QM(DFT)/MM calculations to compare the glycosylation, hydrolysis and transglycosylation steps catalyzed by wild type Thermus thermophilus β-glycosidase (family GH1), a retaining glycosyl hydrolase for which a transglycosylation yield of 36% has been determined experimentally. The three transition states have a strong oxocarbenium character and ring conformations between 4H3 and 4E. The atomic charges at the transition states for hydrolysis and transglycosylation are very similar, except for the more negative charge of the oxygen atom of water when compared to that of the acceptor Glc. The glycosylation transition state has a stronger S N 2 character than the deglycosylation ones and the proton transfer is less advanced. At the QM(PBE0/TZVP)/MM level, the TS for transglycosylation has shorter O4GLC-C1FUC (forming bond) distance and longer OE2GLU338-C1FUC (breaking) distance than the hydrolysis one, although the HACC proton is closer to the Glu164 base in the hydrolysis TS. The QM(SCC-DFTB)/MM free energy maxima show the inverted situation, although the hydrolysis TS presents significant structural fluctuations. The 3-OHGLC group of the acceptor Glc (transglycosylation) and WAT432 (neighbor water in hydrolysis) are identified to stabilize the oxocarbenium transition states through interaction with O5FUC and O4FUC. The analysis of interaction suggests that perturbing the Glu392-Fuc interaction could increase the T/H ratio, either by direct mutation of this residue or indirectly as reported experimentally in the Asn390I and Phe401S cases. The molecular understanding of similarities and differences between hydrolysis and transglycosylation steps may be of help in the design of new biocatalysts for glycan synthesis.
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  • 文章类型: Journal Article
    背景:在这项研究中,我们比较了3种马的母胎界面的糖基化:马,驴和斑马,所有这些都可以杂交产生杂种,评估它们的聚糖相似性和差异。
    方法:从3个马(马)胎盘标本(妊娠50、200和280天)切下的切片,使用抗生物素蛋白-过氧化物酶揭示系统,用一组24种生物素化的凝集素对一头驴(马牛)胎盘(胎冠长度65厘米)和5个斑马(马牛)胎盘标本(妊娠81-239天)进行染色。
    结果:所有三个标本之间的胎儿-母体界面处的凝集素组织化学仅存在微小的定量差异;斑马胎盘表达更多的α2,6连接的唾液酸,在微绒毛界面处具有α1,2岩藻糖基残基。然而,斑马滋养层显示出与其他两个物种的组织学差异,极化的细胞,突出的超核高尔基体,细胞内颗粒较少。
    结论:我们的发现似乎证实了密切相关的假设,与上皮视胎盘的杂交物种在胎儿-母体界面表达相似的聚糖,从而支持胎盘糖编码的存在。我们还观察到种内进化转移与不同的组织学结构和缺乏明显的细胞内颗粒有关。
    BACKGROUND: In this study, we compare glycosylation at the fetomaternal interface in 3 equine species: horse, donkey and zebra, all of which can interbreed to produce hybrids, to assess their glycan similarities and differences.
    METHODS: Sections cut from 3 specimens of horse (Equus caballus) placenta (50, 200 and 280 days gestation), one donkey (Equus asinus) placenta (65 cm crown-rump length) and 5 specimens of zebra (Equus quagga) placentae (81-239 days gestation) were stained with a panel of 24 biotinylated lectins using an avidin-peroxidase revealing system.
    RESULTS: There were only slight quantitative differences in the lectin histochemistry at the feto-maternal interface between all three specimens; zebra placentae expressed more α2,6-linked sialic acid, with α1,2fucosyl residues at the microvillous interface. However, zebra trophoblast showed histological differences from the other two species, with polarised cells, prominent supranuclear Golgi bodies, and fewer intracellular granules.
    CONCLUSIONS: Our findings appear to confirm the hypothesis that closely related, interbreeding species with epitheliochorial placentae express similar glycans at the feto-maternal interface, thereby supporting the existence of a placental glycocode. We also observed intraspecies evolutionary diversion to be associated with a different histological architecture and the absence of significant intracellular granules.
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  • 文章类型: Journal Article
    It is becoming increasingly clear that glycosylation plays important role in intercellular communication within the immune system. Glycosylation-dependent interactions are crucial for the innate and adaptive immune system and regulate immune cell trafficking, synapse formation, activation, and survival. These functions take place by the cis or trans interaction of lectins with glycans. Classical immunological and biochemical methods have been used for the study of lectin function; however, the investigation of their counterparts, glycans, requires very specialized methodologies that have been extensively developed in the past decade within the Glycobiology scientific community. This mini-review intends to summarize the available technology for the study of glycan biosynthesis, its regulation and characterization for their application to the study of glycans in immunology.
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