)沿海拔梯度的基因频率分布

在瑞士阿尔卑斯山的2个定点样地,黄花茅从森林线（海拔1700 m）到山顶（海拔2830 m）呈连续分布。在海拔梯度样带的最高和最低定样场所间的垂直距离差不多为1000 m,但2个定样场所间相距仅仅1.4 km。在所研究的3个海拔梯度样带中,3个同工酶位点（Px-1, Got-2和 Mdh-1）被观察到有统计意义的倾群变异。研究结果显示：沿海拔梯度样带的亚居群间的基因流可能太弱不足以克服自然选择的影响,后者促使对局部环境的适应。在这种情况下,温度因子至少可能作为一种主要的自然选择力起作用。     

阿尔卑斯山黄花茅（Anthoxanthum alpinum）沿海拔梯度的基因频率 …

在瑞士阿尔卑斯山贩２个定点样地,黄花茅从森林线（海拔１７００ｍ）到山顶（海拔２８３０ｍ）呈连续分布。在海拔梯度样带的最高和最低定样场所间的垂直距离差不多为１０００ｍ,但２个定样场所间相距仅仅１．４ｋｍ。在所研究的３个海拔梯度样带中,３个同工酶位点（Ｐｘ－１,Ｇｏｔ－２和Ｍｄｈ－１）被观察到有统计意义的倾群变异。研究结果显示：沿海拔梯度样带的亚居群间的基因流可能太弱不足以克服自然选择的影响,后者促使     

福建梅花山常绿阔叶林植物物种多样性及其海拔梯度格局

常绿阔叶林是福建梅花山国家级自然保护区地带性植被。采用样带与典型群落调查法对区内的常绿阔叶林14400m2样地展开调查,并对植物多样性海拔梯度格局进行分析,结果表明：（1） 群落植物物种丰富度、Gleason丰富度指数、Simpson指数、Shannon Wiener指数和Pielou均匀度指数的均值分别为64.42、10.75、5.75、3.50、0.58,且这5种指数在各样带间差异极为显著,并随海拔的升高均呈单峰曲线变化,峰值出现在海拔700m~900m。（2） 群落各层次的植物物种丰富度、Shannon Wiener指数均呈现灌木层（包括幼树和层间植物）〉乔木层〉草本层的特征。乔木、灌木层物种丰富度与乔木层Shannon Wiener指数在海拔梯度上的样带间差异极显著,变化趋势与群落相似;灌木层与草本层Shannon Wiener指数以及草本层物种丰富度随海拔梯度变化不明显。因此,梅花山自然保护区常绿阔叶林植物物种多样性的海拔梯度格局呈现单峰分布,并支持中间高度膨胀模式（mid domain model）。     

海拔梯度变化对四川西岭雪山小型兽类群落的影响研究

2022年5—10月,利用夹夜法和陷阱法对四川西岭雪山小型兽类群落的海拔梯度变化进行了研究,在海拔1 000～4 600 m设置102个样方,捕获小型兽类32种884只。以400 m海拔梯度分析小型兽类群落：随海拔梯度升高,群落第一优势种形成了从北社鼠Niviventer confucianus（海拔1 000～1 800 m）,转变成中华姬鼠Apodemus draco（海拔1 800～3 400 m）,再到松田鼠属未定名种Neodon sp.（海拔3 400 m以上）的替换现象;物种多样性垂直分布格局为中峰格局,物种丰富度在海拔1 800～3 400 m最高;发现松田鼠属Neodon一新物种,确认壮鼩鼹Uropsilus robustus Wan, 2015新种地位成立。本研究强调了对完整海拔梯度进行全面抽样调查的重要性,从而能够较为客观地反映真实的生物多样性海拔分布格局。     

大兴安岭森林草原过渡带白桦及主要草本植物生态位关系的研究

以白桦、日阴菅及其它主要草本植物的个体数量为指标,分析了各植物种群在土壤有机质,速效P和pH值3个资源维上的生态位宽度和生态位重叠及其在不同海拔条件下的变化规律。日阴菅生态位宽度随海拔升高而增大,其余植物种类在有机质资源维上的生态位宽度,大都是以中等海拔（800m)的样带最宽,而在速效P资源维上,又以中等海拔的样带为最窄,由于高海拔及相应低气温在某种程度上限制了植物种群在土壤有机质和速效P的利用,主要植物种对之间在这两个资源维上的生态位重叠以高海拔（950m)样带为最小,在土壤pH值资源维上,溪荪与其它主要植物种间的生态位重叠皆以低海拔（650m)样带为最小,可能是其特殊的环境组合迫使溪荪发生了生态位移动,大多数种对在土壤有机质,速效P和pH值3个资源维上都以海拔800m的样带生态位重叠最大。     

川西北高原不同海拔高度披碱草与垂穗披碱草核型分析

目的：为研究不同海拔居群染色体核型变异及进化程度,为披碱草的分类及进化研究提供细胞学资料。方法：以川西北高原6个海拔梯度的披碱草居群和5个海拔梯度的垂穗披碱草居群为材料,采用滴片法制片对染色体进行核型分析。结果：披碱草居群D3057（海拔3 057 m）、D2682（海拔2 682 m）的核型公式为2n=6x=42=42m,为1B型;D2384（海拔2 384 m）核型公式为2n=6x=42=42m(4sat),为1A型;D2143（海拔2 143 m）、D1747（海拔1 747 m）的核型公式为2n=6x=42=40m+2sm,为1B型;D1589（海拔1 589 m）的核型公式为2n=6x=42=36m+6sm,为2B型。垂穗披碱草Y2126（海拔4 050 m）、Y2117（海拔3 800 m）、Y2291a(4 150 m)居群的核型公式为2n=6x=42m,ZY3034（海拔3 200 m）的居群核型公式为2n=6x=40m+2M,Y2122（海拔4 800 m）核型公式为2n=6x=40m+2sm,5个居群的核型类型均为1B型。基于核型对称性与进化指数,披碱草居群D158...     

云南大围山种子植物区系海拔梯度格局分析

 海拔梯度包含了多种环境因子的梯度效应,因而研究山地植物区系的海拔梯度格局对揭示植物区系的环境梯度变化规律、了解生物适应性和生物多样性沿海拔梯度的变化趋势等具有重要意义。为了探讨山地植物区系构成特征及其海拔梯度的生态意义,该文根据对大围山国家级自然保护区植被线路调查和垂直样带调查,并结合文献研究等获得的植物区系资料,分析了该保护区种子植物区系构成的基本特征及其随海拔梯度的变化趋势;利用系统聚类的方法寻找和研究大围山植物区系沿海拔梯度变化的断点位置。研究结果表明：1)大围山大多数热带成分分布的上限位于海拔1 500 m左右,以此为界划分热带雨林和常绿阔叶林是合理的。 2)湿润雨林分布于海拔700 m以下;山地雨林分布于海拔700～1 500 m;季风常绿阔叶林分布于海拔1 300～1 800 m;山地苔藓常绿阔叶林分布于海拔1 800 m以上;在海拔2 100 m以上的迎风坡面、土层瘠薄的地段分布有不甚典型的山地苔藓矮林。     

热带森林群落土壤种子库对海拔梯度的响应

在西双版纳海拔800~1400 m的热带森林中,设置海拔梯度垂直样带和样地,研究热带森林群落土壤种子库对海拔梯度的响应。结果发现:(1)土壤种子库的密度和物种丰富度在海拔800 m最大,分别为10540±1578粒·m-2和71个种,最小的土壤种子库密度和物种丰富度则分别出现在海拔1400 m和1200 m。基于Bray-Curtis相似性系数,对4个海拔的土壤种子库物种进行了NMDS排序,发现不同海拔土壤种子库物种组成存在显著的空间分异。(2)土壤种子库中的异质性成分丰富度也因海拔不同存在差异,海拔800 m有9个异质性成分种,海拔1400 m只有5个;而异质性成分种的多度却在海拔1200 m最大。(3)土壤种子库与地上植被的相似性在4个海拔带都低于15%。研究表明,海拔变化对土壤种子库的密度、物种组成格局都能产生显著影响。     

南岭国家级自然保护区森林群落β多样性随海拔梯度的变化

在广东南岭国家级自然保护区海拔300-1900m的范围内,海拔每升高100m设置一条水平样带,共计调查了17条样带,样地面积20400m2。运用相关分析、回归分析和方差分析研究森林群落β多样性随海拔梯度的变化。结果表明:无论是相邻样带还是基准样带,Cody指数以及物种周转速率βC与海拔均呈显著的线性负相关(P<0.05);森林群落各层的共有种数随物种周转速率βC的增加而减少(P<0.05);单因素方差分析及多重比较揭示,Cody指数能较好地反映各层之间物种沿海拔梯度的变化差异。与相异性系数(community dissimilarity)、Bray-Curtis指数和Morisita-Horn指数、以及物种周转速率Sβ和物种周转速率t相比,Cody指数和物种周转速率βC能较好地反映南岭国家级自然保护区森林群落β多样性的海拔梯度格局。     

基于4个线粒体基因的不同海拔高原林蛙群体遗传多样性研究

高原林蛙Rana kukunoris是中国特有的两栖动物,分布于青藏高原海拔2 000～4 400 m的湿润环境。为探究青藏高原的高原林蛙遗传多样性,将4个线粒体基因（COⅠ、cyt b、12S rRNA和16S rRNA）序列合并成联合数据集,对采自青海省4个海拔梯度（2 000 m、2 600 m、3 200 m和3 800 m）的100只高原林蛙个体进行测序分析。结果表明,2 000 m和2 600 m的高原林蛙群体的多态位点、单倍型多样性、核苷酸多样性和平均核苷酸差异数高于3 200 m和3 800 m群体;4个群体均出现了高单倍型多样性、低核苷酸多样性的结果。高原林蛙遗传分化主要发生在群体间,中性检验和错配分析表明,高原林蛙群体可能没有经历扩张事件。cyt b基因在2 600 m、3 200 m和3 800 m群体都检测到了正选择位点。综上所述,2 000 m和2 600 m的高原林蛙群体遗传多样性高于3 200 m和3 800 m群体,4个海拔群体的遗传分化程度较高;cyt b基因可能对高原林蛙适应高海拔环境起到了积极作用。本研究可为理解高原林蛙适应高原环境及其保护提供参考...     

A primordial tRNA modification required for the evolution of life?

The evolution of reading frame maintenance must have been an early event, and presumably preceded the emergence of the three domains Archaea, Bacteria and Eukarya. Features evolved early in reading frame maintenance may still exist in present-day organisms. We show that one such feature may be the modified nucleoside 1-methylguanosine (m(1)G37), which prevents frameshifting and is present adjacent to and 3' of the anticodon (position 37) in the same subset of tRNAs from all organisms, including that with the smallest sequenced genome (Mycoplasma genitalium), and organelles. We have identified the genes encoding the enzyme tRNA(m(1)G37)methyltransferase from all three domains. We also show that they are orthologues, and suggest that they originated from a primordial gene. Lack of m(1)G37 severely impairs the growth of a bacterium and a eukaryote to a similar degree. Yeast tRNA(m(1)G37)methyltransferase also synthesizes 1-methylinosine and participates in the formation of the Y-base (yW). Our results suggest that m(1)G37 existed in tRNA before the divergence of the three domains, and that a tRNA(m(1)G37)methyltrans ferase is part of the minimal set of gene products required for life.     

Peptides corresponding to the second repeated sequence in MAP-2 inhibit binding of microtubule-associated proteins to microtubules

Bovine brain high molecular weight microtubule-associated proteins (MAPs) can be displaced from assembled tubules by peptides corresponding to the second of three nonidentical repeated sequences in mouse MAP-2. The octadecapeptide m2 (VTSKCGSLKNIRHRPGGG) can release MAP-1b from MAP-containing microtubules, and the extended second-sequence peptide m2' (VTSKCGSLKNIRHRPGGGRVK) displaces MAP-1a and MAP-1b as well as MAP-2a and MAP-2b. Peptides m2 and m2' stimulate tubulin polymerization in the absence of MAPs or microtubule-stabilizing agents, and m2' acts as a competitive inhibitor of radiolabeled MAP-2 binding. The dissociation constant for MAP-2 binding to taxol-stabilized tubules was 3.4 microM in the absence of m2' and 14 microM in the presence of 1.5 mM of the m2' peptide. We estimate that the inhibition constant for peptide m2' is about 0.5 mM, about 100 times lower than for the Km of MAP-2. These observations suggest that the second repeated sequence in MAP-2 may represent an important recognition site for MAP binding to microtubules and that other structural features within MAP-2 may reinforce the strength of MAP-microtubule interactions.     

The striatum and cerebral cortex express different muscarinic receptor mRNAs

The existence of four distinct muscarinic acetylcholine receptor genes (m1 – m4) has recently been demonstrated. cDNAs for three of these receptors have been cloned from brain (m1, m3, m4) and one from heart (m2). To gain some understanding of the physiological role of the brain muscarinic receptors, we mapped the distribution of their mRNAs in rat brain by in situ hybridization. These mRNAs are barely detectable in the hindbrain and cerebellum. Within forebrain, each mRNA has a strikingly different pattern of distribution. The highest levels of m1 mRNA are in the cerebral cortex and hippocampus followed by the striatum. m3 mRNA is also prominent in the cerebral cortex, but has very low levels in the striatum. Conversely, the levels of m4 mRNA are highest in the striatum. Since the cognitive effects of muscarinic drugs have been localized to the cerebral cortex and hippocampus, and their psychomotor effects to the striatum, these data suggest that the muscarinic receptors which subserve these responses may be different gene products. Finally, we show that these muscarinic receptors can be distinguished pharmacologically, suggesting that it may be possible to develop drugs for the selective treatment of the psychomotor vs cognitive difficulties of Parkinson's and Alzheimer's disease, respectively.     

运动后尿液蛋白质分子量与等电点的变化特征

通过对９名男性受试者在分别完成１００－２００ｍ,４００－８００ｍ和１ ５００－３ ０００ｍ跑步间歇训练后尿蛋白分子量和等电点的测定发现：①运动时尿液高、低分子量蛋白质排泄率均较运动前明显增加,但以高分子量蛋白质排泄为主;②运动时尿液高、低分子量蛋白质排泄率均以４００－８００ｍ间歇训练时最高,１００－２００ｍ间歇训练时次之,１ ５００－３ ０００ｍ间歇训练时最低;③运动时尿液排出的蛋白质以负离子为主     

Roles for the two 1-butanol dehydrogenases of Pseudomonas butanovora in butane and 1-butanol metabolism

Pseudomonas butanovora grown on butane or 1-butanol expresses two 1-butanol dehydrogenases, a quinoprotein (BOH) and a quinohemoprotein (BDH). BOH exhibited high affinity towards 1-butanol (K(m) = 1.7 +/- 0.2 microM). BOH also oxidized butyraldehyde and 2-butanol (K(m) = 369 +/- 85 microM and K(m) = 662 +/- 98 microM, respectively). The mRNA induction profiles of BOH and BDH at three different levels of 1-butanol, a nontoxic level (0.1 mM), a growth-supporting level (2 mM), and a toxic level (40 mM), were similar. When cells were grown in citrate-containing medium in the presence of different levels of 1-butanol, wild-type P. butanovora could tolerate higher levels of 1-butanol than the P. butanovora boh::tet strain and the P. butanovora bdh::kan strain. A model is proposed in which the electrons from 1-butanol oxidation follow a branched electron transport chain. BOH may be coupled to ubiquinone, with the electrons being transported to a cyanide-sensitive terminal oxidase. In contrast, electrons from BDH may be transferred to a terminal oxidase that is less sensitive to cyanide. The former pathway may function primarily in energy generation, while the latter may be more important in the detoxification of 1-butanol.     

Fine Structure of the Stoma of Bunonema sp. and Teratorhabditis palmarum (Nematoda) and Its Phylogenetic Significance

Fine structure of the stoma, including the cheilostom, gymnostom, and stegostom of Bunonema sp. and Teratorhabditis palmarum was compared with Caenorhabditis elegans to consider fine structural characters that may be phylogenetically informative. The stegostom, enclosed by the anterior end of the pharynx, includes a triradiate lumen surrounded by radial cells (interradial or pairs of adradial cells) repeated in the dorsal and subventral sectors; in Rhabditina, typically the stegostom includes anteriorly two sets of epithelial and posteriorly two sets of muscular radial cells. These muscle cells are anteriorly m1 and posteriorly m2. In Bunonema sp., unlike T. palmarum and C. elegans, the stegostom has a third set of interradial epithelial cells. In Bunonema sp., m1 is expressed by three interradial cells, whereas in T. palmarum and C. elegans m1 is three pairs of adradial muscle cells (i.e., six cells). In all three taxa m2 is expressed as three pairs of adradial muscle cells. Posterior processes of adjacent adradial cells fuse, and closely apposed nuclei may present a figure-eight shape. However, in Bunonema the three interradial m1 cells each have a long posterior process enclosing two separate round nuclei. In combination with additional characters, these diverse stoma features may prove phylogenetically informative. Specifically, the radial epithelial cells of the stegostom appear to be a synapomorphy consistent with a bunonemid-diplogastrid-rhabditid clade, whereas a thickening in the dorsal sector of the stoma cuticle lining is interpreted as a synapomorphy supporting a bunonemid-diplogastrid clade.     

Effects of melatonin on synaptic ribbons in pinealocytes of the Chinese hamster,Cricetulus griseus

Summary The effects of melatonin on synaptic ribbons (SR) in pinealocytes of the Chinese hamster (Cricetulus griseus) were examined. SR were classified into types 1, 2 and 3, which appear as rods, round or irregular bodies and ring-shaped structures, respectively; a synaptic ribbon index (SR index) was determined for the three types. Administration of two doses of 1.5 mg/kg melatonin at noon and 3 p.m. causes an increase in the type-1 and type-2 SR indices 3 h after the second injection in hamsters kept under alternating light and dark conditions (lights on from 7 a.m. to 7 p.m.). Likewise, in animals that are exposed to extended light for 6 h and receive two doses of melatonin at 7 p.m. and 10 p.m., an increase in the type-1 and type-2 SR indices occurs 3 h after the second injection. The increase in the type-2 SR index induced by melatonin administration to hamsters exposed to extended light is greater than the increase in the type-1 SR index under the same experimental conditions. Type-2 SR index, but not type-1 SR index, increases following bilateral superior cervical ganglionectomy. An increase in type-1 and type-2 SR indices occurs at 6 p.m. in ganglionectomized animals administered two doses of melatonin 6 h (noon) and 3 h (3 p.m.) before the time of sacrifice. No significant change is observed in type-3 SR index in animals subjected to any of the above treatments. The results indicate that exogenous melatonin may act directly on pinealocytes of the Chinese hamster to cause an increase in size and/or number of the type-1 and type-2 SR. Type 3-SR may have a role different from that of type-1 and type-2 SR; type-1 and type-2 SR may be functionally related.     

Two distinctive cell binding patterns by vacuolating toxin fused with glutathione S-transferase: one high-affinity m1-specific binding and the other lower-affinity binding for variant m forms

The Helicobacter pylori VacA causes large intracellular vacuoles in epithelial cells such as HeLa or RK13 cells. Two major VacA forms, m1 and m2, divergent in an approximately 300 amino acid segment within the cell binding domain P58, display distinct cell-type specificity. Sequence analysis of four vacA alleles showed that a m1-like allele (61) and two m2 alleles (62 and v226) mainly differed in the midregion and that v225, a m1m2 chimera, was a natural double crossover from v226 and another allele. Each of these alleles was expressed as a soluble GST-VacA fusion that did not form a large oligomer. The recombinant VacA portion nevertheless assembled into higher ordered structures and possessed biological binding activity similar to that of the native VacA. A direct comparison of fusion-cell binding activity showed that m1 > m1m2 > m2 in HeLa cells, whereas there were more similar activities in RK13 cells. Vacuolating analyses of three forms revealed a positive correlation between cell binding activity and vacuolating activity. Moreover, the m1-type N-terminal half portion of the midregion was crucial for HeLa cell cytotoxicity. Kinetic, Scatchard, and inhibition analyses suggested the presence of at least two receptors: a m1-type specific high-affinity receptor (K(d) = approximately 5 nM) and a common VacA receptor interacting similarly with m1, m1m2, and m2 via a lower affinity (K(d) = 45-67 nM). Expression of mainly the m1-type receptor on HeLa cells whereas both receptors on RK13 cells may account for distinct cell binding activity and therefore for cell-type specificity.     

The Yo-Yo intermittent recovery test level 1 is reliable in young high-level soccer players

The aim of the study was to investigate test reliability of the Yo-Yo intermittent recovery test level 1 (YYIR1) in 36 high-level youth soccer players, aged between 13 and 18 years. Players were divided into three age groups (U15, U17 and U19) and completed three YYIR1 in three consecutive weeks. Pairwise comparisons were used to investigate test reliability (for distances and heart rate responses) using technical error (TE), coefficient of variation (CV), intra-class correlation (ICC) and limits of agreement (LOA) with Bland-Altman plots. The mean YYIR1 distances for the U15, U17 and U19 groups were 2024 ± 470 m, 2404 ± 347 m and 2547 ± 337 m, respectively. The results revealed that the TEs varied between 74 and 172 m, CVs between 3.0 and 7.5%, and ICCs between 0.87 and 0.95 across all age groups for the YYIR1 distance. For heart rate responses, the TEs varied between 1 and 6 bpm, CVs between 0.7 and 4.8%, and ICCs between 0.73 and 0.97. The small ratio LOA revealed that any two YYIR1 performances in one week will not differ by more than 9 to 28% due to measurement error. In summary, the YYIR1 performance and the physiological responses have proven to be highly reliable in a sample of Belgian high-level youth soccer players, aged between 13 and 18 years. The demonstrated high level of intermittent endurance capacity in all age groups may be used for comparison of other prospective young soccer players.     

Phosphine-containing HYNIC derivatives as potential bifunctional chelators for (99m)Tc-labeling of small biomolecules

Two prototype phosphine-containing HYNIC chelators, HYNIC-Kp-DPPB and HYNIC-Ko-DPPB (HYNIC = 6-hydrazinonicotinamide; K = lysine; and DPPB = diphenylphosphine-benzoic acid), have been synthesized and characterized by NMR ((1)H, (13)C, and (31)P) and LC-MS. Macrocyclic (99m)Tc complexes, [(99m)Tc(HYNIC-Ko-TPPB)(tricine)] and [(99m)Tc(HYNIC-Kp-DPPB)(tricine)], were prepared by reacting the phosphine-containing HYNIC chelator with (99m)TcO(4)(-) in the presence of excess tricine and stannous chloride. Results from this study clearly demonstrated that both HYNIC-Kp-DPPB and HYNIC-Ko-DPPB are able to form highly stable macrocyclic (99m)Tc complexes, [(99m)Tc(HYNIC-Ko-TPPB)(tricine)] and [(99m)Tc(HYNIC-Kp-DPPB)(tricine)], when tricine is used as the coligand. Radio-HPLC data suggest that the complex [(99m)Tc(HYNIC-Kp-DPPB)(tricine)] exists as only one detectable isomer in solution while the complex [(99m)Tc(HYNIC-Ko-DPPB)(tricine)] has three isomers. It was also found that three isomers of [(99m)Tc(HYNIC-Ko-DPPB)(tricine)] interconvert at elevated temperatures, suggesting that the presence of these isomers might be due conformational changes in the macrocyclic Tc chelate. The LC-MS data for both macrocyclic (99m)Tc complexes are completely consistent with the proposed composition. The phosphine-containing HYNIC chelators described in this study may have the potential as bifunctional chelators for (99m)Tc labeling of small biomolecules.