基于景观尺度下的鄱阳湖湿地浅层土有机碳的空间特征

湿地土壤有机碳研究是全球碳循环研究的基础性工作, 对于准确评估湿地固碳增汇和全球温室气体减排都具有重要意义。以鄱阳湖国家自然保护区为研究区域, 选择六种景观类型(湿地洲滩景观包括受人工控制的碟形湖泊常湖池、半人工控制的碟形湖泊蚌湖、不受人工控制的洲滩前缘泗洲头以及岗地景观包括林地、田地和菜地), 湿地洲滩景观在各1 m高程(泗洲头和蚌湖采样高程10-17 m, 常湖池采样高程12-17 m)内的浅土壤采取3个土壤样品, 岗地景观浅层土壤各采取3个土壤样品, 分析浅层土壤有机碳含量。结果表明, 鄱阳湖不同景观类型的浅层土壤有机碳含量差异性显著。湿地洲滩浅层土壤(特别是0-10 cm土层)的有机碳随高程梯度变化呈现倒U型变化, 即低海拔与高海拔土壤有机碳的含量较中海拔土壤有机碳的含量低, 泗洲头洲滩土层0-10 cm的有机碳含量最高值出现在13-14 m高程, 其中0-10 cm土层的土壤有机碳含量变化值为1.56-12.29 g·kg-1, 10-20 cm土层的土壤有机碳含量变化值为0.96-8.19 g·kg-1; 蚌湖洲滩土层0-10 cm的有机碳含量最高值出现在14-15 m高程, 其中0-10 cm土层的土壤有机碳含量变化值为6.36-23.32 g·kg-1, 10-20 cm土层的土壤有机碳含量变化值为4.14-8.88 g·kg-1; 常湖池洲滩土层0-10 cm的有机碳含量最高值出现在16-17 m高程, 其中0-10 cm土层的土壤有机碳含量变化值为6.51-18.91 g·kg-1, 10-20 cm土层的土壤有机碳含量变化值为3.83-10.05 g·kg-1。岗地浅层土壤有机碳(特别是0-10 cm土层)田地的土壤有机碳含量最高, 菜地土壤有机碳含量最低。比较六种景观类型的浅层土壤有机碳含量, 泗洲头洲滩浅层土壤有机碳含量最低, 蚌湖洲滩浅层土壤有机碳含量最高。六种景观类型的浅层土壤有机碳含量呈现一致的现象是土层0-10 cm的机碳含量明显高于土层10-20 cm的有机碳含量, 说明鄱阳湖国家自然保护区内土壤有机碳含量主要富集在土壤浅层的特征。土壤pH值对湿地土壤有机碳呈显著负相关性, 而土壤含水量、地上部分生物量与土壤有机碳呈显著正相关性。     

人正常腺上皮组织中MUC6基因的表达

应用免疫组织化学和原位杂交方法检测人正常腺上皮中MUC6基因的表达,揭示MUC6基因在正常人腺上皮组织中的分布异质性及其特点.结果显示MUC6基因编码的核心蛋白及其mRNA主要分布于正常胃粘膜胃腺的基底部,上皮细胞无MUC6基因表达,呈细颗粒状,位于细胞核周,胃底、胃窦的表达无区别;十二指肠绒毛上皮内的表达呈弥漫性,均质状,杯状和柱状细胞的表达类似,杯状细胞的粘液滴内未测得MUC6基因产物;空肠、结肠组织中无MUC6基因的表达;胆囊上皮组织内有强阳性MUC6核心蛋白的表达,而宫颈上皮中表达较弱.实验提示MUC6基因的表达存在异质性及器官特异性.     

青蛤的营养成分分析与评价

测定了61、2月份青蛤(Cyclina sinensis)的营养成份,并对其营养价值进行综合评定。结果表明,6月份青蛤的营养较12月份好,其粗蛋白比12月的高出2.84%,粗脂肪含量高出1.74%;6月和12月的氨基酸总含量分别为826.3 mg/g蛋白质和804.0 mg/g蛋白质,其中必需氨基酸分别占36.1%和33.6%,氨基酸计分(AAS)和化学评分(CS)是6月的较高,必需氨基酸指数(EAAI)则分别为64.23和59.88。其不饱和脂肪酸占脂质总量的67.7%,其中单烯酸占24.9%,多烯酸占42.8%,“脑黄金”DHA和EPA的含量分别达到11.3%和18.4%。还含有多种微量元素和维生素。     

Effects of electrical stimulation in vivo of M. pectoralis on carbohydrate metabolism with reference to certain liver and blood values in the pigeon

The pectoralis muscles of two groups of anaesthetized pigeons were exercised in vivo by electrical stimulation for periods of 1 h and 5 h respectively. There was no significant change from controls in the level of blood glucose in both groups. Blood lactate level was significantly higher in the exercised groups but was relatively lower in the 5-h control group in comparison with its 1-h counter part. Blood lactate dehydrogenase (LDH) activity was significantly higher in the 1-h stimulated pigeons as was also the case with liver LDH in the same group but markedly lower in the 5-h ones. No significant change was seen in liver glycogen content in the stimulated pigeons. Liver phosphorylase activity was markedly low in the 5-h stimulated pigeons as was also the case with liver LDH activity. Circulating level of corticosterone was significantly higher in both the stimulated groups. Blood thyroxine (T4) as well as triiodothyronine (T3) levels were considerably reduced in both stimulated groups. The T3/T4 ratio was higher in the 5-h stimulated pigeons. It was concluded that, while initially carbohydrate was used as fuel for exercise, in prolonged exercise, lipid became the chief fuel as was shown in earlier studies. While fat continued to be used as the main fuel, carbohydrate was spared and also gluconeogenesis was enhanced. It was also concluded that the r?le of the thyroid hormones in promoting oxidative metabolism was enhanced by markedly increasing peripheral deiodination of T4 to T3 in prolonged exercise.     

粗柄独尾草不同器官蒽醌类成分的消长规律

采用高效液相色谱法对沙生类短命植物粗柄独尾草苗期、营养生长期、初花期、盛花期、果期各器官中大黄素、大黄酚、大黄酸、芦荟大黄素含量的消长规律进行了研究。结果表明:叶中,芦荟大黄素的含量在苗期和初花期都较高,在盛花期时最低;大黄酸的含量在苗期最高,盛花期时最低;大黄素的含量在苗期达到最高,初花期和盛花期最低;大黄酚的含量也以苗期最高,盛花期和果期最低。且在初花期时,4种蒽醌类物质含量均呈现明显的叶先端>叶中部>叶基部的空间差异性。根中,芦荟大黄素的含量在苗期和营养生长期较高,而以盛花期和果期较低;大黄酸的含量在果期最高,其余时期差异不显著;大黄素的含量以苗期和初花期较高;大黄酚的含量在果期达最高,而盛花期时最低。同时期的根叶蒽醌含量相比,叶中的芦荟大黄素要高于根,而根中大黄酚含量要高于叶。同时期各器官蒽醌总量相比:叶>根>花>花葶。故若选取粗柄独尾草作为蒽醌类药材利用,建议最佳采集方式为采集初花期的叶先端部分。     

Change in Hatching Enzyme Activity during Development of the Sea Urchin, Hemicentrotus Pulcherrimus

The time course of change in hatching enzyme activity during development of embryos of the sea urchin Hemicentrotus pulcherrimus was observed. The enzyme was present in the particulate fraction in embryos until the time of hatching and was maximal at the time of hatching. Cell fractionation studies suggested the existence of an inhibitor of the hatching enzyme. This possibility was subsequently substantiated by experiments in mixtures of fractions: the activity of hatching enzyme in the particulate fraction was inhibited by the supernatant of embryos. This inhibitory factor was heat-stable and non-dialyzable, but it was not characterized further. The activity of secreted hatching enzyme was not inhibited by this factor, suggesting that the molecular forms of hatching enzyme in embryos and in the culture supernatant are different. After hatching, the amount of increase in the hatching enzyme activity in the culture supernatant was 3.5 times the amount of decrease in enzyme activity in the embryos, suggesting that the enzyme was activated during its secretion.     

Flower-inducing and -inhibiting activities of Phloem Exudate from Cotyledons of Pharbitis Seedlings

The flower-inducing and -inhibiting activities of phloem exudate (PE) prepared from cotyledons of Pharbitis seedlings were examined, using apex cultures in vitro from Pharbitis as a bioassay system.The PE was prepared from photoperiodically-induced cotyledons (SD-PE). The SD-PE was subjected to the following fractionations: When the SD-PE was extracted with CHCl₃ and then ethyl acetate, the inducing activity was located in the final aqueous fraction. The activity was localized in the diffusate when the aqueous fraction was dialyzed (molecular weight cut off was 10,000). The diffusate was fractionated by ion exchange chromatography, and flower-inducing activity was found in the fraction adsorbed onto anion exchange resin. When the fraction was applied to a Sep-Pak C18 cartridge, the activity eluted with 25% MeOH. As a result of the above fractionation, activity was increased about 30-fold.The nature of the flower-inhibiting activity of the PE taken from cotyledons exposed to continuous-light conditions was examined (CL-PE). The inhibiting activity was decreased as the cotyledons were exposed to longer dark periods; it appeared to be heat-stable. The CL-PE also inhibited flowering in Lemna. The CL-PE was subjected to the following fractionations: When the CL-PE was extracted with CHCl₃ and ethyl acetate, activity was located in the final aqueous fraction. Activity was localized in the diffusate when the aqueous fraction was dialyzed (molecular weight cut off was 10,000). When the diffusate was fractionated by ion exchange chromatography, the activity was found in the flow-through fraction. When the fraction was applied to a hydroxyapatite cartridge, the activity eluted with 25 mM sodium phosphate buffer. When the fraction was re-dialyzed (molecular weight cut off was 1,000), the diffusate contained the activity. As a result of the above fractionation, activity was increased about 10-fold.     

深圳地铁碳排放量

本文从列车牵引用电和地铁站场用电两方面分析了深圳地铁的碳排放量。首先,计算出深圳地铁2008年牵引用电量为2514万度,2009年为2635万度;地铁站场2008年的用电量为1.08亿度,2009年为1.12亿度。其次,根据南方电网单位电力碳排放量计算出深圳地铁2008年的碳排放量为28053.695吨,旅客人均耗电量为0.984度,旅客人均碳排放量207.025克;2009年为碳排放量28572.561吨,旅客人均耗电量为1.002度,旅客人均碳排放量206.697克。然后,与深圳公交、出租车和香港地铁进行了比较。2008年,由于运量客较少,深圳地铁的旅客人均碳排放量,约为出租车的46%,是深圳公交大巴的1.99倍、中巴的1.26倍。此外,深圳地铁的旅客人均耗电量与香港地铁大致相当,由于香港地铁所用电力的碳排放较低,使得深圳地铁旅客人均碳排放量是香港地铁的1.24倍。最后,对2012年深圳地铁的碳排放进行了预测。结果显示,2012年,深圳地铁的碳排放总量将可能增加9.32倍。客运量约为11.62-7.26亿人次,相应地,旅客人均碳排放量将增加10.86-77.39%。     

正常人及肝细胞癌患者肝脏及血浆中丙酮酸激酶同工酶免疫测定

 分别从人肝及鼠肝中高度纯化L型和M_1型丙酮酸激酶(Pyk),制备相应的免抗血清。从抗血清中纯化IgG并水解成F(ab')_2,进而还原成Fab',后者与辣根过氧物酶(HRP)交联成Fab'-HRP,再利用这两种复合物建立了各自的高灵敏夹心ELISA来免疫定量L及M_2型(与鼠M_1-Pyk有交叉免疫)Pyk,结果发现:正常人肝中95％的Pyk为L型,M_2-Pyk仅占5％,而肝细胞癌中L-Pyk降至正常肝的3.5％,M_2-Pyk却增至正常的14.6倍,以致M_2-Pyk占总量的95.5％。免疫组化研究进一步证实定量的结果,正常人肝L-Pyk染色呈强阳性。M_2-Pyk染色较弱,而肝细胞癌恰好相反,L-Pyk染色明显减退,而M_2-Pyk不仅癌组织染色很深,癌周组织也明显深于正常,而且愈近癌巢,染色愈深。测定血浆Pyk,发现正常人L-Pyk占89.9％,M-Pyk(以M_2计)仅占10.1％。肝细胞癌患者血浆L-Pyk略见降低,为正常值的79.6％,p值在0.02～0.05之间,但血浆M型Pyk明显升高至正常的4.59倍,占Pyk总量的39.6％,并证明主要来源于肝癌组织中的M_2,故M_2-Pyk有可能成为肝细胞癌诊断的新指标。     

不结球白菜叶子重量性状遗传模型分析

应用主基因+多基因6个世代联合分离分析方法, 对不结球白菜SI×秋017组合的叶片重和叶柄重性状进行了分析。结果表明, SI×秋017组合的叶片重性状遗传受1对负向完全显性主基因+加性-显性多基因(D-4)控制, 主基因加性效应为1.8991, 显性效应为-1.8991; 多基因加性效应为-1.2934, 显性效应为1.7933; 势能比值为-1.3865, 显性度为-1.0000; B1、B2和F2世代群体叶片重的主基因遗传率分别为6.98%、4.33% 和36.08%; B1、B2和F2世代群体叶片重的多基因遗传率为16.03%、7.39%和23.96%。叶柄重的遗传受1对加性主基因+加性-显性多基因(D-2)控制, 主基因加性效应为-1.1457, 显性效应为0; 多基因加性效应为1.3472, 多基因显性效应为2.5788; 势能比值为1.9142, 显性度为0。B1、B2和F2世代群体叶柄重的主基因遗传率分别为31.72%、5.27%和57.94%。B1、B2和F2世代群体叶柄重的多基因遗传率分别为0.42%、4.59%和4.80%。对SI×秋017组合叶片重性状的改良要在晚代选择; 对叶柄重的改良要以主基因为主, 可在早代选择。     

云南丽江山慈菇遗传多样性的DALP分析

采用DALP (Direct amplification of length polymorphism) 分子标记技术, 对产自云南的药用植物丽江山慈菇Iphigenia indica (L.) Kunth的9个居群进行DNA指纹检测。筛选出5个引物组合, 扩增共产生131条DNA片段, 其中104 条谱带具有遗传多态性, 约占79 39%, 平均每组引物扩增所得多态条带为20 8, 9个居群平均多态百分率为42 21%。9个居群平均观察等位基因数Na为1 4224, 总Na为1 7939; 平均有效等位基因数Ne 为1 3141, 总Ne 为1 4810; 平均遗传多样性指数H为0 1745, 总H为0 2831; 平均Shannon 多样性指数I 为0 2527, 总I为0 4231; 总基因多样性Ht为0 2831, 居群内多样性Hs 为0 1745, 居群间基因分化系数Gst为0 3834, 即丽江山慈菇有61 66%的遗传变异来自居群内, 38 34%来自居群间, 居群间存在较高水平的遗传分化。滇西北居群的遗传多样性明显高于滇中居群的遗传多样性, 这与滇中地区丽江山慈菇野生资源被大规模挖掘有着直接的关系。     

Endogenous beta-galactoside-binding lectin expression is suppressed in retinol-induced mucous metaplasia of chick embryonic epidermis

The fate of endogenous beta-galactoside-binding lectin of chick embryo (14K type) was investigated during the course of skin differentiation. Lectin (14K) was found in keratinized epidermis and was localized mainly in the basal and intermediate cells. However, the protein lectin in the epidermis disappeared when the cultured skin was treated with vitamin A and mucous metaplasia was observed. The synthesis of lectin mRNA was also strongly suppressed by vitamin A in a concentration-dependent manner. On the other hand, in the dermis, in which the lectin was localized in the extracellular matrix, lectin expression was scarcely affected by vitamin A. These results indicated that the lectin was expressed in the keratinized epidermis but that its expression was suppressed in vitamin A-induced mucous-secreting epithelium. The suppression may be a result of a transition of the epidermal regulatory system to one of mucous-secreting epithelium. This is the first finding that 14K lectin expression might be regulated during the course of the epidermal differentiation.     

Marginal bone loss around axial and straight implants supported with prefabricated SFI-Bar with mandibular overdentures

To assess the role of prefabricated SFI-Bar in peri-implant bone loss around immediately axially loaded and straight implants. This study comprised of 40 complete denture wearer patients who received two axially parallel implants connected by SFI-Bars in group I and two 15° mesially tilted implants connected by SFI-Bars in group II. Peri- implant bone loss (PiBL) was measured at 1 year, 2 years and 3 years. The mean PiBL at 1 year in group I was 0.21 mm and I group II was 0.22, at 2 years in group I was 0.26 mm and in group II was 0.23 mm and at 3 years, in group I was 0.29 mm and in group II was 0.34 mm. The difference was significant at 3 years (P< 0.05). The mean mesial PIBL at 1 year in group I was 0.18 mm, in group II was 0.20 mm, at 2 years in group I was 0.19 mm and in group II was 0.07 mm and at 3 years, in group I was 0.25 mm and in group II was 0.29 mm. The difference found to be significant in each time duration in both groups (P< 0.05).The mean distal PIBL at 1 year in group I was 0.23 mm, in group II was 0.22 mm, at 2 years in group I was 0.33 mm and in group II was 0.39 mm and at 3 years, in group I was 0.34 mm and in group II was 0.39 mm. The difference found to be significant at 2 and 3 years in both groups (P< 0.05). Authors found that mandibular overdentures retained with Prefabricated SFI-Bar with axial and straight inserted implants may be useful in patients with reduced bone height.     

Lactic acid extraction with trioctyl amine

Lactic acid extraction was carried out with trioctyl amine (TOA) in three diluents. The effect of initial lactic acid concentrations on the extraction efficiency was investigated. It was observed that although the percentage extraction remained constant or decreased but the loading ratio was increased in all the cases. The overloading was observed in the case of TOA in methyl isobutyl ketone (MIBK). The extraction of lactic acid was favored at a lower aqueous pH?in all the diluents. The improvement of the extraction efficiency at a higher aqueous pH?(=?6) was achieved by using the modified TOA (treated with HCl) in MIBK. However, the recovery of lactic was very poor in the case of modified TOA in MIBK, although the complete recovery was obtained for untreated TOA.     

The Influence of Feeding and Oral Rehydration on the Bioavailability of Oxytetracycline in Calves

The influence of feeding on the bioavailability of oxytetracycline was studied in preruminant calves. Oxytetracycline was given in water as a drench to fasting calves or was mixed in the milk replacer. Compared to water the bioavailability was significantly reduced (53.5%) when oxytetracycline was mixed in the milk re-placer. A further reduction, 83.3 %, occurred when the calves were treated one hour post milk feeding. Also concentrate was found to reduce the bioavailability. Very high serum levels were recorded when the drug was given in an oral rehydration solution, pH 4.9, containing glycine. The values obtained when an alkaline (pH 8.3) solution without glycine was used did not differ from the levels recorded when oxytetracycline was given in water. It was suggested that the use of oxytetra-cyclines in feeds may be questioned because of their well-known complex forming ability.     

Distribution of isotopic label after the oral administration of free and bound 14C-labelled glucosamine in rats

The metabolic fate of [1-(14)C]glucosamine, of N-acetyl[1-(14)C]glucosamine and of glycoproteins labelled with [1-(14)C]glucosamine was studied in rats for a period of 24hr. after these materials were given orally or injected. When [1-(14)C]glucosamine was injected 26.3% of the label was excreted in the urine, 19.7% was expired as carbon dioxide and 12.7% was incorporated into plasma proteins. When the same compound was given orally, 49.2% of the label was expired as carbon dioxide, with little appearing in the urine or in the plasma. When N-acetyl[1-(14)C]glucosamine was injected, 51.3% of the label was excreted in the urine with 12.3% appearing in carbon dioxide, but there was little incorporation into plasma protein. When this compound was given orally, 46.5% of the label was expired as carbon dioxide, 7.4% was recovered in the urine and 1.7% was incorporated into plasma protein. After the injection of (14)C-labelled glycoprotein 21.0% of the label was expired as carbon dioxide, whereas when it was given orally 49.8% of the label was recovered in carbon dioxide. The differences observed between the metabolic fate of the amino sugars when they were given orally and their fate when injected could not be accounted for by the action of the intestinal microflora or by the rate of administration of the material. It is concluded that amino sugars undergo metabolic alteration or degradation during absorption.     

Phospholipase activities in subcellular fractions of human platelets.

A homogenate of human platelets was fractionated by zonal ultracentrifugation into membranes, various granules and mitochondria. The membrane fraction was composed of two populations. The first, which represented 75% of the proteins, was rich in plasma membranes; the second, which represented the remaining 25%, was rich in microsomal membranes. Lysophospholipase was essentially localised in the cytosol. Phospholipase A1 which was only weakly bound to membranes, was mostly found in the soluble fraction (75%); the remainder was located in the plasma membranes and the mitochondria. Two-thirds of the phospholipase A2 was found in the particulate fractions.     

Analysis of Nuclear Accumulation of Influenza Nucleoprotein Antigen in the Presence of p-Fluorophenylalanine

When p-fluorophenylalanine (FPA) was added to influenza virus RI/5+-infected cells 4 hr after infection, virus-specific proteins were synthesized but infectious progeny virus was not produced. In these cells, synthesis of viral RNA was strongly inhibited and nucleoprotein (NP) antigen was found predominantly in the nucleus in contrast to untreated cells in which NP antigen was distributed throughout the whole cell. The intracellular location and migration of NP were examined by isotope labeling followed by fractionation of infected cells. In untreated cells, a large portion of the NP was present in the cytoplasm and most of it was detected in the form of ribonucleoprotein (RNP). In contrast, in FPA-treated cells little viral RNP was detectable and NP was present predominantly in the nucleus in a nonassembled, soluble form. When FPA was removed from the culture, synthesis of viral RNA was soon restored and a large amount of viral RNP appeared in the cytoplasm; this was followed by the production of infectious virus. The results of the experiments suggest that the NP synthesized in the presence of FPA is not assembled into viral RNP because of the lack of available RNA, and such NP migrates readily into the nucleus and accumulates there.     

Estrogen metabolism in hyperthyroidism and in cirrhosis of the liver.

Estrogen metabolism was studied in spontaneous hyperthyroidism (Graves disease) and in alcoholic cirrhosis of the liver. The plasma concentration of estradiol-17beta (PCE2) was increased in men with hyperthyroidism. Although the metabolic clearance rate of estradiol-17beta (MCRE2) was reduced, the production rate (PR) of the steroid was increased above normal. The MCRE2 was also decreased in women with hyperthyroidism but the PCE2 and PRE2 was unchanged from normal. The conversion ratio of estradiol-17beta (CRE2E1) was increased in both hyperthyroid men and women. The PCE2 was significantly increased in men with cirrhosis of the liver. The MCRE2 was normal and this resulted in an increase in the PRE2 in this disorder. The CRE2E1 was significantly higher than normal. The plasma concentration of estrone (E1) was elevated in men with both disorders.