Scolopendra subspinipes mutilans protected the ceruleininduced acute pancreatitis by inhibiting high-mobility group box protein-1

AIM:To evaluate the inhibitory effects of Scolopendra subspinipes mutilans(SSM) on cerulein-induced acute pancreatitis(AP) in a mouse model.METHODS:SSM water extract(0.1,0.5,or 1 g/kg) was administrated intraperitoneally 1 h prior to the first injection of cerulein.Once AP developed,the stable cholecystokinin analogue,cerulein was injected hourly,over a 6 h period.Blood samples were taken 6 h later to determine serum amylase,lipase,and cytokine levels.The pancreas and lungs were rapidly removed for morphological examination,myeloperoxidase assay,and real-time reverse transcription polymerase chain reaction.To specify the role of SSM in pancreatitis,the pancreatic acinar cells were isolated using collagenase method.Then the cells were pre-treated with SSM,then stimulated with cerulein.The cell viability,cytokine productions and high-mobility group box protein-1(HMGB-1) were measured.Furthermore,the regulating mechanisms of SSM action were evaluated.RESULTS:The administration of SSM significantly attenuated the severity of pancreatitis and pancreatitis associated lung injury,as was shown by the reduction in pancreatic edema,neutrophil infiltration,vacuolization and necrosis.SSM treatment also reduced pancreatic weight/body weight ratio,serum amylase,lipase and cytokine levels,and mRNA expression of multiple inflammatory mediators such as tumor necrosis factor-α and interleukin-1β.In addition,treatment with SSM inhibited HMGB-1 expression in the pancreas during AP.In accordance with in vivo data,SSM inhibited the cerulein-induced acinar cell death,cytokine,and HMGB-1 release.SSM also inhibited the activation of c-Jun NH2-terminal kinase,p38 and nuclear factor(NF)-κB.CONCLUSION:These results suggest that SSM plays a protective role during the development of AP and pancreatitis associated lung injury via deactivating c-Jun NH2-terminal kinase,p38 and NF-κB.

Antihepatoma peptide,scolopentide,derived from the centipede scolopendra subspinipes mutilans

BACKGROUND Centipedes have been used to treat tumors for hundreds of years in China.However,current studies focus on antimicrobial and anticoagulation agents rather than tumors.The molecular identities of antihepatoma bioactive components in centipedes have not yet been extensively investigated.It is a challenge to isolate and characterize the effective components of centipedes due to limited peptide purification technologies for animal-derived medicines.AIM To purify,characterize,and synthesize the bioactive components with the strongest antihepatoma activity from centipedes and determine the antihepatoma mechanism.METHODS An antihepatoma peptide(scolopentide)was isolated and identified from the centipede scolopendra subspinipes mutilans using a combination of enzymatic hydrolysis,a Sephadex G-25 column,and two steps of high-performance liquid chromatography(HPLC).Additionally,the CCK8 assay was used to select the extracted fraction with the strongest antihepatoma activity.The molecular weight of the extracted scolopentide was characterized by quadrupole time of flight mass spectrometry(QTOF MS),and the sequence was matched by using the Mascot search engine.Based on the sequence and molecular weight,scolopentide was synthesized using solid-phase peptide synthesis methods.The synthetic scolopentide was confirmed by MS and HPLC.The antineoplastic effect of extracted scolopentide was confirmed by CCK8 assay and morphological changes again in vitro.The antihepatoma effect of synthetic scolopentide was assessed by the CCK8 assay and Hoechst staining in vitro and tumor volume and tumor weight in vivo.In the tumor xenograft experiments,qualified model mice(male 5-week-old BALB/c nude mice)were randomly divided into 2 groups(n=6):The scolopentide group(0.15 mL/d,via intraperitoneal injection of synthetic scolopentide,500 mg/kg/d)and the vehicle group(0.15 mL/d,via intraperitoneal injection of normal saline).The mice were euthanized by cervical dislocation after 14 d of continuous treatment.Mechanistically,flow cytometry was conducted to evaluate the apoptosis rate of HepG2 cells after treatment with extracted scolopentide in vitro.A Hoechst staining assay was also used to observe apoptosis in HepG2 cells after treatment with synthetic scolopentide in vitro.CCK8 assays and morphological changes were used to compare the cytotoxicity of synthetic scolopentide to liver cancer cells and normal liver cells in vitro.Molecular docking was performed to clarify whether scolopentide tightly bound to death receptor 4(DR4)and DR5.qRT-PCR was used to measure the mRNA expression of DR4,DR5,fas-associated death domain protein(FADD),Caspase-8,Caspase-3,cytochrome c(Cyto-C),B-cell lymphoma-2(Bcl-2),Bcl-2-associated X protein(Bax),x-chromosome linked inhibitor-of-apoptosis protein and Cellular fas-associated death domain-like interleukin-1βconverting enzyme inhibitory protein in hepatocarcinoma subcutaneous xenograft tumors from mice.Western blot assays were used to measure the protein expression of DR4,DR5,FADD,Caspase-8,Caspase-3,and Cyto-C in the tumor tissues.The reactive oxygen species(ROS)of tumor tissues were tested.RESULTS In the process of purification,characterization and synthesis of scolopentide,the optimal enzymatic hydrolysis conditions(extract ratio:5.86%,IC_(50):0.310 mg/mL)were as follows:Trypsin at 0.1 g(300 U/g,centipede-trypsin ratio of 20:1),enzymolysis temperature of 46°C,and enzymolysis time of 4 h,which was superior to freeze-thawing with liquid nitrogen(IC_(50):3.07 mg/mL).A peptide with the strongest antihepatoma activity(scolopentide)was further purified through a Sephadex G-25 column(obtained A2)and two steps of HPLC(obtained B5 and C3).The molecular weight of the extracted scolopentide was 1018.997 Da,and the peptide sequence was RAQNHYCK,as characterized by QTOF MS and Mascot.Scolopentide was synthesized in vitro with a qualified molecular weight(1018.8 Da)and purity(98.014%),which was characterized by MS and HPLC.Extracted scolopentide still had an antineoplastic effect in vitro,which inhibited the proliferation of Eca-109(IC_(50):76.27μg/mL),HepG2(IC_(50):22.06μg/mL),and A549(IC_(50):35.13μg/mL)cells,especially HepG2 cells.Synthetic scolopentide inhibited the proliferation of HepG2 cells(treated 6,12,and 24 h)in a concentration-dependent manner in vitro,and the inhibitory effects were the strongest at 12 h(IC_(50):208.11μg/mL).Synthetic scolopentide also inhibited the tumor volume(Vehicle vs Scolopentide,P=0.0003)and weight(Vehicle vs Scolopentide,P=0.0022)in the tumor xenograft experiment.Mechanistically,flow cytometry suggested that the apoptosis ratios of HepG2 cells after treatment with extracted scolopentide were 5.01%(0μg/mL),12.13%(10μg/mL),16.52%(20μg/mL),and 23.20%(40μg/mL).Hoechst staining revealed apoptosis in HepG2 cells after treatment with synthetic scolopentide in vitro.The CCK8 assay and morphological changes indicated that synthetic scolopentide was cytotoxic and was significantly stronger in HepG2 cells than in L02 cells.Molecular docking suggested that scolopentide tightly bound to DR4 and DR5,and the binding free energies were-10.4 kcal/mol and-7.1 kcal/mol,respectively.In subcutaneous xenograft tumors from mice,quantitative real-time polymerase chain reaction and western blotting suggested that scolopentide activated DR4 and DR5 and induced apoptosis in SMMC-7721 Liver cancer cells by promoting the expression of FADD,caspase-8 and caspase-3 through a mitochondria-independent pathway.CONCLUSION Scolopentide,an antihepatoma peptide purified from centipedes,may inspire new antihepatoma agents.Scolopentide activates DR4 and DR5 and induces apoptosis in liver cancer cells through a mitochondria-independent pathway.

WUGONG MTS.REGION AS A CALEDONIAN MEDIUM-HIGH PRESSURE METAMORPHIC BELT:EVIDENCE FROM b_0 VALUES OF WHITE MICAS

The Wugong Mts. region may have experienced three stages of metamorphism in Early Paleo-zoic, which may be closely related to the generations of regional deformation. The first stage ismedium-pressure metamorphism, the second medium- and high-pressure one with stress on high-pressure metamorphism, and the third low-pressure and high-temperature metamorphism. Theregion, as a whole, is a Caledonian medium-high pressure metamorphic belt.

STAT3 Inhibition by Centipede Scolopendra Extract in Liver Cancer HepG2 Cells and Orthotopic Mouse Models of Hepatocellular Carcinoma

Objective To observe the effects of Centipede Scolopendra extraction(CSE)on human liver cancer HepG2 cells and the nude mouse tumor model of liver orthotopic transplantation,and to explore the anti-liver cancer mechanism of the extract.Methods HepG2 cells were respectively treated with CSE250(250μg/mL),CSE500(500μg/mL)and 5-FU,and control group was established.An enzymatic hydrolysis and acetone precipitation method was used to separate and purify CSE,which was then used to treat HepG2 cells.The CCK8 assay was used to detect the inhibition of cell proliferation and the half maximal inhibitory concentration(IC50)was calculated.Flow cytometry was used to analyze the cell cycle,and western blot was used to detect the expression of signal transduction and activator of transcription 3(STAT3)pathway-related proteins in HepG2 cells treated with CSE.A nude mouse model with an orthotopic liver tumor was prepared.The mice were randomly divided into four groups,each containing 12 animals:the model group,the 5-FU group,the CSE10 group[10 mg/(kg·d)]and the CSE50 group[50 mg/(kg·d)].The volume and mass changes in the nude mice with orthotopic transplanted tumors were observed.Western blot method was used to test the protein expression levels of p-STAT3 and p38 mitogen-activated protein kinase(p38MAPK).Tissues from the liver of mice in the model group and the CSE50 group were analyzed by using a protein tyrosine kinase(PTK)chip,and the Gene Ontology(GO)and Kyoto Encyclopedia of Genes and Genomes(KEGG)function enrichment analysis of the differentially expressed proteins was performed.Results This study showed that CSE significantly inhibited the proliferation of HepG2 cells(P<0.05).After 48 h of CSE treatment,the cell cycle of HepG2 cells manifested as S phase and G2/M phase;p-STAT3 protein levels in the CSE groups were significantly lower than that in the control group(P<0.05).Analysis of the tumor inhibition in the mice showed that the tumor masses and volume in CSE groups were lower(P<0.05).The protein levels of p-STAT3 and p38MAPK in CSE50 group and 5-FU group decreased significantly(P<0.05).PTK antibody chip screening results showed that CSE groups had a bidirectional regulation trend,and there were 23 up-regulated PTKs and six down-regulated PTKs.The GO and KEGG analyses showed that CSE exerted its anticancer effects through regulation of biological processes,including mitogen-activated protein kinase(MAPK)cascade,chemotaxis,cell invasion,cell adhesion,angiogenesis and other biological processes,and through signaling pathways,including the MAPK,phosphatidylinositol-3-kinase/serine threonine protein kinase(PI3K/AKT),and RAS signaling pathways.Conclusions CSE can effectively inhibite the proliferation of HepG2 cells and effectively inhibite the growth of liver cancer orthotopic transplantation tumor.Its mechanism may be closely related to the regulation of STAT3,MAPK and PI3K/AKT signaling pathways.

全域旅游视域下武功山辐射区域“三生空间”格局优化研究

规划农业文化旅游“三位一体”“三产融合”“三生同步”对形成区域联动下旅游品质提升具有重要的现实意义。文章探究2000年、2010年和2020年江西武功山辐射区域“三生空间”格局演变趋势,结合政策导向进行格局优化设计。研究发现:(1)构建辐射区域土地利用转移矩阵,整体格局由生态空间转入生产空间明显,部分生产、生态空间转出为复合型生活空间,生态空间受到社会经济与可持续政策影响呈波动变化。(2)分析空间结构动态转换剧烈程度,尤其以生产、生活空间最为突出,生态空间综合动态度波动较为稳定,但生态空间与生产、生活空间转移关系仍需协调。(3)辐射区域格局演变以原始生态格局为语境,受到品质旅游需求、政策规划方向、区域供需体系构建因素的主要影响,而人文历史名迹为潜在韧性因素持续存在。研究认为武功山辐射区域发展需聚焦于空间属性协调共生、人地关系相互制约、提升游客旅游与居民生活幸福感,进而保障辐射区域空间刚性,逐步修正以引导空间秩序趋向稳定。

蜈蚣败毒饮联合肤舒止痒膏治疗寻常型银屑病血热风燥型的临床疗效及对免疫因子CXCL9、CXCL10的影响

目的:观察蜈蚣败毒饮联合肤舒止痒膏治疗寻常型银屑病血热风燥型的临床疗效,以及对免疫相关因子CXCL9、CXCL10的影响。方法:选取黑龙江中医药大学附属第一医院皮肤科2021年5月—2023年5月就诊的寻常型银屑病血热风燥型患者72例,随机分为治疗组与对照组,每组36例。试验中脱落6例,最终治疗组35例,给予口服蜈蚣败毒饮联合外用肤舒止痒膏治疗,对照组31例,仅口服消银胶囊治疗。记录治疗前、治疗后第2周和第4周的皮损面积和严重程度指数(PASI)、皮肤病生活质量指数(DLQI)、中医证候评分进行差异性比较,并检测外周血中CXCL9和CXCL10含量。结果:两组治疗后第2、4周PASI评分、DLQI评分和中医证候评分均明显低于治疗前,且治疗组患者明显低于对照组,差异均有统计学意义(P<0.05)。两组血清中CXCL9和CXCL10含量大幅度下降(P<0.05),且治疗组趋化因子含量远低于对照组(P<0.05)。结论:蜈蚣败毒饮联合肤舒止痒膏能有效改善皮肤病变状况及症状,提升患者生活质量,且安全性高,适合临床推广使用。

蜈蚣药材、饮片、标准汤剂与配方颗粒的特征图谱相关性研究及量值传递分析

目的建立蜈蚣药材、饮片、标准汤剂与配方颗粒的高效液相色谱(HPLC)特征图谱,并测定其中次黄嘌呤、苯丙氨酸成分的含量,考察四者之间化学成分的传递与差异。方法采用Dikma Platisil ODS-C18(250 mm×4.6 mm,5μm)色谱柱,以甲醇和水为流动相梯度洗脱,流速为1 mL·min^(-1),柱温为25℃。以含量、特征图谱共有峰传递数及相似度为主要评价指标,分析其量值传递规律。结果18批蜈蚣药材、饮片、标准汤剂及3批配方颗粒特征图谱均有8个共有特征峰,与各自对照特征图谱相似度均大于0.90,指认出尿嘧啶、酪氨酸、次黄嘌呤、黄嘌呤、苯丙氨酸、肌苷、鸟苷、色氨酸8种成分,并测定其含量,未出现离散数据。结论蜈蚣药材、饮片、标准汤剂与配方颗粒的主要化学成分基本相同,HPLC特征图谱相关性良好,8种成分在测定范围内与峰面积线性关系良好。所建立质量评价模式能够反映蜈蚣4种形态多成分的整体面貌,为蜈蚣配方颗粒质量控制提供数据支撑。

非物质文化遗产视域下武功土织布产业现代化发展

文章概述了陕西省武功县土织布产业现代化转型的进展,通过调研发现其存在产品单一、品质低、缺乏品牌及集群效应等问题。为此,建议明确发展目标、加强产销体系建设、加大产品创新力度、推动产业集群发展,以推动产业现代化转型,促进地方经济持续发展,并传承弘扬非遗文化,助力乡村振兴。

共情视域下跨界景区旅游文创产品开发与设计——以江西武功山为例

跨界旅游区作为一种特殊的地理空间,因行政边界区划使其被割裂为具有不同发展特征的景区空间。跨界景区间品牌共享从一定程度上推动了其合作的深入,但其本位发展意识仍从一定程度上造成旅游消费市场的隐性流失。故为谋求跨界景区间更大的共利空间,尝试依托共情理论,依托旅游文创产品这一跨界旅游生产要素,围绕景区和游客“品牌共享—感知共情—产品共创—认知共情—利益共生—行为共情”互动共情过程及价值实现路径,结合“走遍、走进、最爱”武功山三大共情层次,分别提出武功山旅游数字纪念章、旅游吉祥物、旅游纪念礼品等旅游文创产品的设计理念,以期推动其整体旅游格局的真正实现。

网络关注度视角下武功山露营旅游需求时空特征及其影响因素研究

基于百度指数平台,获取2011至2021年武功山露营旅游搜索指数,利用季节性结构分量模型和空间地理分析等方法,探究武功山露营旅游网络关注度时空分布规律及其影响因素,结论表明:时间分布特征上,网络关注度水平整体呈现逐年增长态势,仅2020至2021年间小幅下降,季节变化上呈现“双峰”和“多峰”特征,季节性差异显著,在“五一”和“十一”假期中,关注度集中分布在假期前段;空间分布特征上,全国范围内分布不均匀,存在地域差异,华中地区关注度水平最高,东北地区关注度水平最低,且空间距离越远网络关注度水平越低;影响因素上,经济发展水平、互联网发达程度、森林覆盖率与武功山露营网络关注度呈现显著正相关,空间地理距离与网络关注度呈现显著的负相关。基于以上分析,课题组提出优化武功山露营旅游网络关注度时空分布的四条措施。

黑头蜈蚣的化学成分

本文报道了黑头蜈蚣Scolopendra negrocapitis化学成分,并与中国药典收载的少棘巨蜈蚣S.subspinipes mutilans进行了比较。黑头蜈蚣含总脂18.7％,蛋白质63.4％,游离氨基酸11.9％;含有与少棘巨蜈蚣相同的12种脂肪酸(其中不饱和脂肪酸占64％),21种氨基酸和12种微量元素;蛋白质聚丙酰胺凝胶电泳分离出14条色带。表明黑头蜈蚣与少棘巨蜈蚣主要化学成分类同,是一种值得开发利用的新药源。

多棘蜈蚣化学成分的研究

目的：分析多棘蜈蚣（ＳｃｏｌｏｐｅｎｄｒａｍｕｌｔｉｄｅｎｓＮｅｗｐｏｒｔ）的化学成分，并与药典收载品少棘蜈蚣（Ｓ．ｍｕｔｉｌａｎｓＬ．Ｋｏｃｈ）比较。方法：采用溶媒提取法测定总脂，气相色谱质谱计算机检测脂肪酸，微量凯氏定氮法测定蛋白质，离子交换色谱测定游离氨基酸，电感耦合离子发射光谱测定微量元素。结果：多棘蜈蚣含总脂７．２％，蛋白质６４．６％，游离氨基酸６．３％；含有与少棘蜈蚣相同的１５种脂肪酸（其中不饱和脂肪酸占７２％）、２１种氨基酸和１２种微量元素。结论：多棘蜈蚣与少棘蜈蚣主要化学成分类同，某些成分含量存在差异，是一种值得开发利用的药用蜈蚣资源。

全蝎蜈蚣对CIA大鼠外周血CD4^+CD25^+FoxP3^+Treg细胞的调节

目的:观察全蝎蜈蚣对胶原免疫性关节炎(Collagen-Induced Arthritis,CIA)大鼠外周血CD4+CD25+FoxP3+Treg细胞的调节作用。方法:Wistar大鼠60只,随机分成6组,分别为正常对照组、模型对照组、全蝎蜈蚣高(0.4 g/kg)、中(0.2 g/kg)、低剂量(0.1 g/kg)组和Ⅱ型胶原蛋白(60μg/kg)治疗组(CⅡ组),二型胶原蛋白诱导大鼠关节炎,并采用流式细胞术检测大鼠外周血CD4+CD25+FoxP3+Treg细胞及酶联免疫吸附试验检测血清中IL-2表达水平。结果:与模型组比较,全蝎蜈蚣高、低剂量组大鼠外周血CD4+CD25+T细胞及CD4+CD25+FoxP3+Treg细胞水平显著升高,且中、低剂量组血清IL-2水平显著下降。结论:全蝎蜈蚣治疗关节炎大鼠可能是通过上调外周CD4+CD25+FoxP3+Treg细胞表达水平以恢复或重建免疫耐受而实现的。

海拔及旅游干扰对武功山山地草甸土壤渗透性的影响

土壤渗透能力是影响土壤侵蚀的重要因素之一,是反映土壤水源涵养及调节功能的重要指标,目前对于亚热带山地草甸土壤渗透性方面研究较少。江西武功山草甸是亚热带山地草甸的典型代表,以面积广和分布基准海拔低的特点,在华东植被垂直带谱中具有典型性和特殊性,但是人为干扰和过度旅游开发使武功山脆弱的山地草甸出现严重退化和破碎化态势。以武功山不同海拔及旅游干扰程度山地草甸土壤为研究对象,分别测定0—20 cm和20—40 cm土层土壤的初渗率、稳渗率、平均入渗率、前60分钟渗透总量、温度、湿度、容重、最大持水量、最小持水量、毛管持水量、pH、有机质、速效氮、速效磷、速效钾等理化指标,分析不同海拔及干扰程度草甸土壤渗透性特征,探讨影响土壤渗透性的相关因子,为亚热带地区退化草甸的修复及可持续经营提供参考。结果表明:(1)1600—1800 m范围,随着海拔升高,土壤渗透性呈降低趋势,在1900 m范围土壤渗透性又有所提高,各海拔土壤渗透性排序为1600 m>1700 m>1900 m>1800 m。(2)随着干扰程度增强,草甸土壤渗透性呈降低趋势,各干扰程度的土壤渗透性排序为无干扰>轻度干扰>中度干扰>重度干扰。(3)所有草甸分布区0—20 cm土层的土壤渗透性均高于20—40 cm土层,初渗率>平均入渗率>稳渗率。(4)通用经验模型更适合武功山草甸土壤水分入渗过程,Horton模型次之,Philip模型和Kostiakov模型拟合效果都比较差。(5)土壤渗透性与土壤湿度、毛管持水量呈显著正相关(P<0.05),与容重呈显著负相关(P<0.05),初渗率及平均入渗率与速效氮含量显著正相关(P<0.05),稳渗率、平均入渗率、渗透总量与速效钾含量呈显著正相关(P<0.05)。

少棘蜈蚣纤溶活性蛋白的抗血栓作用

目的研究少棘蜈蚣(Scolopendra subspinipes mutilans L.Koch)纤溶活性蛋白的抗血栓作用。方法采用离子交换层析和分子筛等制备法从少棘蜈蚣中纯化到蜈蚣纤溶酶(Scolopendra subspinipes mutilans L.Koch fibrinolyti cenzyme,SSFE),用纤维蛋白平板检测酶活力,常规方法检测了SSFE溶血性和出血性,进行了SSFE体外溶栓和体内溶栓实验,并检测了凝血酶原时间(PT)、活化部分凝血酶时间(APTT)和凝血酶时间(TT)3个标准化指标。结果PAGE显示SSFE为单一组分,具有纤溶活性;证明SSFE无致出血性且无致溶血活性,低、中、高剂量SSFE使小鼠APTT和TT均明显延长,中剂量SSFE对PT有延长作用,而高剂量作用不明显。结论蜈蚣纤溶酶具有抗血栓作用。

蜈蚣有效成分抗心肌缺血作用的研究

目的 :观察蜈蚣有效成分对心肌缺血鼠自由基的变化 ,阐明蜈蚣治疗冠心病的机制。方法 :将4 0只小鼠随机分为 4组 ,A组为空白对照组 ,B组为模型组 ,C组为蜈蚣小剂量 ( 2 5g/kg)治疗组 ,D组为蜈蚣大剂量 ( 5g/kg)治疗组。造模前治疗组用不同剂量的蜈蚣提取物 ,分别按每天 0 2mL/ 1 0g灌胃 ,连续 7天 ,其余两组用等量蒸馏水灌胃。后采用脑垂体后叶素 2 0u/kg腹腔注射 ,诱发心肌缺血。缺血 2 0min后 ,观察各组心肌酶、自由基的变化 ,以及心肌透射电镜。结果 :模型组LDH、MDA明显升高 ,SOD、NO水平显著降低 ,治疗组SOD、NO含量显著提高 ,LDH、MDA明显降低 ,超微结构显示心肌细胞损害明显减轻。且蜈蚣大剂量较小剂量治疗组作用更加明显。结论 :蜈蚣具有抗心肌缺血的作用。

墨江蜈蚣与少棘蜈蚣的比较研究──Ⅰ．化学组成

本文对墨江蜈蚣（ＳｃｏｌｏｐｅｎｄｒａｍｏｊａｎｇｉｃａＺｈａｎｇｅｔＣｈｉ）与少棘蜈蚣（ＳｃｏｔｏｐｅｎｄｒａｓｕｂｓｐｉｎｉｐｅｓｍｕｔｉｌａｎｓＬ．Ｋｏｃｈ）的水分、灼烧残渣、蛋白质、游离氨基酸、微量元素和挥发性脂肪酸的含量进行了系统的测定并比较了两者间的异同性。实验结果表明：墨江蜈蚣的蛋白质、灼烧残渣、水分的含量分别为６７．２％、３．９５％和３．５９％，而少棘蜈蚣分别为６８．８％、４．８０％和３．６５％，它们的含量基本相同。游离氨基酸、挥发性脂肪酸和微量元素的相对含量也很接近，但脂类和总糖的含量差异较大。

基于TM NDVI的武功山山地草甸植被覆盖度时空变化研究

以江西省武功山山地草甸为研究区,基于4期TM(Thematic Mapper,专题测图仪)卫星遥感影像,提取NDVI(Normalized Difference Vegetation Index,归一化植被指数),采用像元二分模型,运用ENVI 5.1和Arc GIS 10.0软件计算得到武功山山地草甸的植被覆盖度分布格局及动态变化。研究结果表明:(1)研究期间山地草甸面积减少了9.72%,呈递减趋势。20年来随着武功山风景区成立—旅游业发展—山地草甸生态修复,山地草甸植被覆盖度增加和减少交替,总体呈上升趋势;(2)山地草甸植被覆盖度呈现东南高西北低的空间分布特征。低覆盖度草甸区集中在武功山山脉的西北侧坡面的崖壁和部分山脊线上,而高覆盖度草甸区多分布在武功山山脉的东南坡面;(3)研究区山地草甸退化与改善并存,山地草甸最北端和白鹤峰-九龙山区域的东南坡、南坡低海拔处植被总体呈退化特征;发云界南部的东坡植被总体呈现改善特征。研究期间山地草甸退化面积比改善面积多出1.78%。(4)山地草甸植被覆盖度的分布格局和地形因子存在较高的相关性(P<0.05):植被覆盖度随着坡向的变化而呈规律性的变化,总体上山地草甸植被覆盖度的分布为阳坡>平坡>阴坡;植被覆盖度先是随着坡度的上升而升高,在坡度15°—25°时达到峰值,然后随坡度的上升而下降,在45°—90°最低;植被覆盖度随海拔升高呈波浪式下降,1000—1200m最高,在主峰山顶海拔1800—1918.3m最低。遥感解译检验结果证明采用此方法对大面积山地草甸覆盖度分布及变化进行反演可行而准确;在后续研究中将采用不同季相的多期影像数据提取NDVI对研究区植被覆盖度进行长期监测,以便更准确可靠地分析山地草甸演化过程和趋势。

武功山山地草甸土壤全量氮磷钾分布格局及对不同退化程度的响应

以武功山核心景区主峰金顶海拔1 600-1 900m之间的自然未退化草甸土壤与1 850m不同退化强度草甸斑块土壤2类处理为研究对象,对其A（0-20cm）、B（20-40cm）2层土壤全氮、全磷、全钾进行测定,分析武功山草甸土全氮、全磷、全钾的分布格局,及武功山草甸土壤全氮、全磷、全钾含量对草甸不同退化程度的响应。结果表明：1）武功山自然状态下草甸土壤全氮、全磷和全钾含量的变化范围分别为2 094.4-7 473.6mg·kg^-1、0.59-1.73g·kg^-1和18.25-54.25g·kg^-1。在同一垂直土壤剖面中均随着发生层的降低而减少,而全钾含量无此特征,且在A、B 2层中差距较小。2）海拔高度的变化对武功山草甸土壤全氮和全磷含量的影响不显著,但是全钾随着海拔的上升呈显著上升趋势。3）不同草甸退化程度对武功山草甸土壤全磷全钾含量的影响不显著,但对全氮含量的影响达到差异显著水平,武功山退化草甸土壤的磷、钾素养分供应水平无较大缺失,但氮素的供应出现明显损失,可为生态修复中调节土壤肥力提供理论指导。

少棘蜈蚣毒液溶血肽的分离纯化

采用超滤和HPLC(包括凝胶过滤层析、阳离子交换层析和反相HPLC)等技术对少棘蜈蚣毒液进行分离纯化,最终获得一个多肽;运用基质辅助激光解吸附飞行时间质谱测定其分子量为4484Da,测得其对小鼠红细胞半数溶血剂量HD50=14.69μg/ml。