红托竹荪菌托多糖的提取及抗肿瘤活性的初步研究

红托竹荪菌托经热水提取、酒精沉淀、脱蛋白后的粗多糖,其得率远大于其菌丝体和子实体的其他部位及香菇子实体。菌托粗多糖进一步用DEAE纤维素柱和Sephadex G-75分离纯化,得到两个组分DRVP1与DRVP2,对分离得到的主要多糖通过高效液相色谱（HPLC）、红外光谱（IR）等进行结构分析。DRVP1的相对分子质量（Mr）为1．47x10^4,红外光谱数据显示为β-型甘露糖苷。体外试验表明,红托竹荪菌托多糖的组分DRVP1对小鼠S180肉瘤有一定的抑制作用。     

红托竹荪菌托多糖的提取及抗肿瘤活性的初步研究

红托竹荪菌托经热水提取、酒精沉淀、脱蛋白后的粗多糖,其得率远大于其菌丝体和子实体的其他部位及香菇子实体.菌托粗多糖进一步用DEAE纤维素柱和Sephadex G-75分离纯化,得到两个组分DRVP1与DRVP2,对分离得到的主要多糖通过高效液相色谱(HPLC)、红外光谱(IR)等进行结构分析.DRVP1的相对分子质量(Mr)为1.47×104,红外光谱数据显示为β-型甘露糖苷.体外试验表明,红托竹荪菌托多糖的组分DRVP1对小鼠S180肉瘤有一定的抑制作用.     

红托竹荪菌托多糖提取工艺及抗氧化降血糖活性

为利用红托竹荪菌托,采用酶解法提取菌托多糖,优化多糖提取工艺,并测定多糖分子量、单糖组成、抗氧化及降血糖活性。结果表明,最佳酶解法提取工艺为纤维素酶2.5%、果胶酶0.4%、木瓜蛋白酶1.5%,50 ℃酶解1 h,料液比1:60、提取温度80 ℃、时间3 h,该条件下多糖提取率达15.37%,比热水浸提法提高39.60%。酶解法多糖分子量为3 344 Da (Mn)、522 208 Da (Mw)、2 929 Da (Mp),主要由葡萄糖、甘露糖、葡萄糖醛酸、半乳糖和岩藻糖等组成,葡萄糖占最高,达48.82%。菌托多糖为2.0 mg/mL时,DPPH·清除率为93.83%,Fe³⁺还原能力为0.140 7,α-葡萄糖苷酶活性抑制率为54.62%、α-淀粉酶活性抑制率为56.45%,与热水浸提法相比差异极显著或显著。酶解法提取红托竹荪菌托多糖,提取率较高,具有较高的抗氧化、降血糖活性,具有推广应用价值。     

红托竹荪多糖对大鼠酒精性肝损伤的保护作用

研究红托竹荪多糖(Dictyophora rubrovalvata polysaccharide,DRP)对酒精所致大鼠肝损伤的保护作用.采用苯酚-硫酸法测得DRP的含量为74.68％±1.32％,利用傅里叶红外光谱初步分析表明DRP是含有α-糖苷键和β-糖苷键的吡喃环多糖.当DRP浓度达到3.0 mg/mL时,DPP...     

棘托竹荪菌托抑菌物质提取、分离及活性组分

以棘托竹荪(Dictyophora echinovolvata)菌托为研究对象,提纯菌托提取物有效抑菌天然产物,分析其抑菌活性组成。选择最佳提取溶剂及指示菌,采用色谱层析法分离纯化,GC-MS检测分析活性组分。结果表明:乙酸乙酯提取物对金黄色葡萄球菌、枯草芽孢杆菌、大肠杆菌、蜡状芽孢杆菌、标准摩根氏菌、肠炎沙门氏菌均有较好的抑制效果;以金色葡萄球菌为指示菌,乙酸乙酯提取物的抑菌作用对温度、紫外线均有较好的稳定性;对提取物进行分离,获得2个有抑菌活性组分DEVⅠ、DEVⅡ,采用GC-MS分析DEVⅠ、DEVⅡ中的化学组分,DEVⅠ中相对含量1%以上的成分有20个;DEVⅡ中相对含量在1%以上成分6个,其中具有抑菌活性的成分为2-呋喃甲酸和肉桂酸,相对含量分别为25.6%和54.2%,推测可能为棘托竹荪菌托抑菌物质的主要组成成分。     

棘托竹荪菌托抑菌物质提取、分离及活性组分北大核心CSCD

以棘托竹荪(Dictyophora echinovolvata)菌托为研究对象,提纯菌托提取物有效抑菌天然产物,分析其抑菌活性组成。选择最佳提取溶剂及指示菌,采用色谱层析法分离纯化,GC-MS检测分析活性组分。结果表明:乙酸乙酯提取物对金黄色葡萄球菌、枯草芽孢杆菌、大肠杆菌、蜡状芽孢杆菌、标准摩根氏菌、肠炎沙门氏菌均有较好的抑制效果;以金色葡萄球菌为指示菌,乙酸乙酯提取物的抑菌作用对温度、紫外线均有较好的稳定性;对提取物进行分离,获得2个有抑菌活性组分DEVⅠ、DEVⅡ,采用GC-MS分析DEVⅠ、DEVⅡ中的化学组分,DEVⅠ中相对含量1%以上的成分有20个;DEVⅡ中相对含量在1%以上成分6个,其中具有抑菌活性的成分为2-呋喃甲酸和肉桂酸,相对含量分别为25.6%和54.2%,推测可能为棘托竹荪菌托抑菌物质的主要组成成分。     

红托竹荪多糖诱导肿瘤细胞凋亡的作用初探

探讨红托竹荪多糖对小鼠腹水瘤S180细胞凋亡的作用。分别使用不同浓度的红托竹荪多糖处理S180细胞24h,Western blot法检测Bcl-xl、Bax、caspase-9和Caspase-3等蛋白表达,使用流式细胞仪检测细胞凋亡。Western blot 法检测结果显示Bcl-xl表达量随竹荪多糖剂量增加而降低,Bax表达量则相反,每组Bax/Bcl-xl的比值增加,Caspase-9、Caspase-3表达量增加;流式细胞仪检测结果显示：0、25、50和100mg/L组细胞凋亡率分别为5.12%±0.11%、9.61%±0.61%、16.39%±0.19%和17.05%±0.13%,与对照组相比细胞凋亡率增高,差异具有统计学意义（P<0.05）,推断红托竹荪多糖具有诱导S180细胞凋亡的功能。     

金针菇子实体多糖分离纯化及结构和免疫活性研究

从金针菇子实体中分离纯化多糖,并对多糖结构和体外免疫活性进行研究。采用水提醇沉法从金针菇子实体中提取粗多糖,利用DEAE-Cellulose-52及Sephacryl S-300HR柱层析纯化得到FVPⅠ-a,再利用HPLC-ELSD技术、红外及核磁共振对FVPⅠ-a进行结构解析。在体外以促RAW264.7巨噬细胞产NO、分泌细胞因子,促进小鼠淋巴细胞增殖实验,考察FVPⅠ-a增强免疫的能力。从金针菇子实体中分离纯化得到FVPⅠ-a,其为分子量81.4kDa,由葡萄糖、果糖和鼠李糖组成的β构型的吡喃型杂多糖。体外免疫实验表明,FVPⅠ-a能够促进RAW264.7巨噬细胞产生NO及分泌细胞因子（IL-1β,IL-6,TNF-α）,能单独的促进小鼠淋巴细胞增殖（P<0.05）,并能协同增强ConA和LPS对小鼠淋巴细胞的促增殖作用（P<0.01,P<0.05）。首次从金针菇子实体中获得FVPⅠ-a杂多糖,其在体外具有增强非特异性免疫反应及增强特异性免疫反应的能力。     

鬼笔属3种真菌的个体发育及形态观察

为揭示鬼笔属真菌子实体各器官的发育过程和形态特点,采用石蜡切片法对驯化栽培出菇的超短裙竹荪Phallus ultraduplicatus、冬荪P. dongsun和红托竹荪P. rubrovolvatus不同发育阶段的菇蕾进行切片显微观察,结合菌丝、孢子和子实体形态比较3个种的个体发育及形态特点。结果表明：3个种的菌丝和孢子形态差异不明显,超短裙竹荪子实体的菌裙质地较薄、长约4 cm、带有不规则形状的网孔;红托竹荪的菌裙质地较厚、长约7 cm、带有圆形网孔;冬荪仅有1层薄菌幕。3个种的菇蕾内部发育顺序一致,最先发育的都是胶质腔,接着是子实层、菌柄腔、菌盖、菌柄、菌裙（菌幕）;发育过程中菌丝形态经历从疏松到紧密、从交织状到组织状的变化过程;各器官发育完成的时间不同,在菇蕾直径相同的条件下,冬荪发育最快,在菇蕾直径为2 cm时,各器官基本发育完成,红托竹荪在菇蕾直径为3 cm时发育完成,超短裙竹荪的菇蕾发育最慢,在直径达到4 cm时各器官才能发育完成。为鬼笔类真菌的分类研究和亲缘关系探索提供了依据。     

苦楝果多糖的分离纯化及组成分析

利用水提醇沉法提取苦楝果实中的多糖,经DEAE-52柱层析分离,得到MP1、MP2和MP3三个多糖组分,用Sephadex G-100凝胶色谱柱对MP1进行纯化鉴定,结果显示为单一峰。借助气质联用仪,对苦楝粗多糖和组分MP1进行了成分分析。红外光谱分析表明苦楝多糖的单糖残基以吡喃环和呋喃环的形式存在。     

小鼠腹腔巨噬细胞被S-O_2-I菌苗激活后的抑瘤作用——Ⅱ.小鼠腹腔巨噬细胞被动转移的抑瘤效应及其肿瘤的病理观察

众所周知肿瘤的发展受宿主免疫功能的影响,当机体免疫功能下降时,肿瘤发展快,死亡率也高。卡介苗和厌氧棒状杆菌苗等一类的细菌佐剂能提高机体的免疫功能,增强机体对肿瘤细胞的排斥能力,它们的抗肿瘤活性和临床应用已有大量报道(Cross et al.,1976;Yamamura et al.,1979;Woodruff et al.,1975;Isral et al.,1976)。近年来,发现S-O_2-1菌苗在临床试用中,具有一定的抗肿瘤活性,并且副作用小,因     

C_(60)对小鼠S_(180)肉瘤光动力学作用模型的建立

为验证Ｃ６０对活体肿瘤的光动力学损伤作用,我们从两方面进行实验：Ｃ６０对荷瘤小鼠的Ｓ１８０实体瘤的光动力学杀伤作用和Ｃ８０对离体Ｓ１８０肿瘤细胞的光动力学杀伤作用,在小鼠的瘤体上注射Ｃ８０光敏剂,在５１１ｎｍ、５７８ｎｍ混合黄录色激光照射正派主发Ｃ６０,产生大量的单线态氧,杀伤活性肿瘤。激光光强为５００ｍＷ,Ｃ６０浓度为３０μｇ／ｍｌ时,荷瘤小鼠寿命平均延长５天,瘤径减小１ｃｍ,瘤重减轻０．８克,     

橙盖鹅膏多糖(AC-1)体外免疫调节活性、细胞毒性和抗肿瘤活性的研究

为研究橙盖鹅膏多糖的体外免疫调节活性、细胞毒性和抗肿瘤活性,本研究运用细胞学技术探究AC-1对T细胞、B细胞和RAW264.7三种免疫细胞的体外免疫调节活性;研究AC-1对小鼠成纤维细胞(L929)的细胞毒性以及对小鼠胃癌细胞(MFC)、小鼠肉瘤细胞(S180)的体外抗肿瘤活性。结果表明,AC-1能在体外显著刺激三种免疫细胞的增殖及RAW264.7细胞的吞噬,表明AC-1在增强机体免疫方面具有重要作用,进一步研究发现AC-1主要通过显著促进IgE和IgG的分泌来增强体液免疫。在浓度为5~20μg/mL时AC-1对L929细胞无显著的促进及抑制作用,说明AC-1对正常细胞无毒性;在浓度为10~20μg/mL时AC-1能显著抑制小鼠胃癌细胞(MFC)的生长,但对小鼠肉瘤细胞(S180)的抑制效果较弱,说明AC-1在体外能够直接抑制肿瘤细胞的生长,但对不同的肿瘤细胞具有不同的抑制效果。综上所述,橙盖鹅膏多糖(AC-1)在体外具有良好的免疫调节活性、抗肿瘤活性,但对不同的肿瘤细胞具有不同的抑制效果并且对正常细胞无毒性。     

Study of cell killing and morphology on S180 by ultrasound activating hematoporphyrin derivatives

Sonodynamic therapy (SDT) is one of antitumor strategies that kill tumor cells through the synergistic effects caused by the combined use of HpD and US[1]. SDT is based on the following principle. Ultrasound used in SDT can penetrate the deep tissue and activate HpD, which accu- mulated in tumor cell, and produce highly active oxygen species[2] such as singlet oxygen (1O2), which can destroy the structure of tumor cells. So far the studies on the SDT have focused mainly on the mechan…     

Study of cell killing and morphology on S180 by ultrasound activating hematoporphyrin derivatives

The inhibition of ascitic S180 and induced sarcoma 180 in vivo was studied with the combination of hematoporphyrin derivatives (HpD) and ultrasound (US) at the frequency of 1.1 MHz and different intensities by light microscopy observation, electronic microscopy observation, cytochemical analysis and fluorescence labeling. The present study indicated that the injury of ascitic S180 increased as time passed and the inhibitory effect was stronger in US plus HpD group than that in other groups. Our results also indicated that the changes in cell structure, cytochrome C oxidase activity, the degradation and missing of DNA were the important factors that inhibited the tumor cell growth and even induced celldeath. The phenomenon of apoptosis of tumor cells indicated that cell death andinduced apoptosis exist in the treatment of sonodynamic therapy (SDT). Our study investigated the mechanism underlying the killing effect of S180 induced by USactivating HpD by the observation of cell morphology and dynamic changes from seminal injury to succeeded injury even to death. It would provide rich referencefor the study of SDT.     

Superoxide dismutase induces G1‐phase cell cycle arrest by down‐regulated expression of Cdk‐2 and cyclin‐E in murine sarcoma S180 tumor cells

As an efficient reactive oxygen species–scavenging enzyme, superoxide dismutase (SOD) has been shown to inhibit tumor growth and interfere with motility and invasiveness of cancer cells. In this study, the molecular mechanisms of cell cycle arrest when S180 tumor cells were exposed to high levels of SOD were investigated. Here, both murine sarcoma S180 tumor cells and NIH‐3T3 mouse fibroblasts were respectively treated with varying concentrations of Cu/Zn‐SOD for 24, 48 and 72 h to determine optimal dose of SOD, which was a concentration of 800 U/ml SOD for 48 h. It is found that SOD induced S180 cell cycle arrest at G1‐phase with decreasing level of superoxide production, whereas SOD had less effect on proliferation of NIH‐3T3 cells. Moreover, the expression rate of Proliferating Cell Nuclear Antigen (PCNA) in S180 tumor cells was suppressed after SOD treatment, which indicated the inhibition of DNA synthesis in S180 cells. Besides, there were significant down‐regulations of cyclin‐E and Cdk‐2 in S180 cells after SOD treatment, which contributed to the blockage of G1/S transition in S180 cell cycle. Together, our data confirmed that SOD could notably inhibit proliferation of S180 tumor cell and induce cell cycle arrest at G1‐phase by down‐regulating expressions of cyclin‐E and Cdk‐2. Copyright © 2012 John Wiley & Sons, Ltd.     

层粘连蛋白糖肽对实体型瘤细胞粘着于层粘连蛋白基质的影响

 本文报告由小鼠EHS瘤提取的层粘连蛋白(Laminin,LN)经链霉蛋白酶(Pronase)消化,再经Sephadex-G50层析分离得到LN总糖肽。它可显著抑制黑色素瘤细胞B16-MBK及S180肉瘤细胞与LN基质的识别及粘着,并具有明显剂量依赖性。与五肽(YIGSR),卵清蛋白及其糖肽,胎球蛋白及其糖肽比较,LN总糖肽的抑制效果显著高于YIGSR及胎球蛋白糖肽,而其它三者均无抑制作用。因而提示:LN分子中一定结构的糖链特异地参与了LN对肿瘤细胞表面LN受体的识别与结合。     

Immunomodulation and antitumor activities of different-molecular-weight polysaccharides from Porphyridium cruentum

The extracellular polysaccharides (EPSs) isolated from Porphyridium cruentum were degraded by hermetical-microwave and H₂O₂ under ultrasonic waves. Six products were obtained with molecular weights of 6.53, 256, 606, 802.6, 903.3 and 1002 kDa. The antitumor and immunomodulatory activities of different-molecular-weight (MW) polysaccharides were evaluated by the S180-tumor-bearing mouse model in vivo and peritoneal macrophage activation in vitro. The degraded EPSs all showed clear immunomodulation to different extents. The MW of the EPSs had a notable effect on their activity. The 6.53-kDa fragment had the strongest immunoenhancing activity. Different doses of EPS all inhibited the growth of the implanted S180 tumor. The tumor inhibition index at high, middle and low doses was 53.3%, 47.5% and 40.5%, respectively. In addition, three different concentrations of EPS significantly increased lymphocyte proliferation, which indicated the unique mechanism of the antitumor effect of EPS.