中国麦红吸浆虫(双翅目：瘿蚊科)不同地理种群的遗传结构

采用RAPD方法测定分析了我国麦红吸浆虫Sitodiplosis mosellana (Gehin) 10个地理种群的遗传结构。结果表明：5种引物在10个种群中共产生了326个RAPD标记,各地理种群之间没有产生各自的特征标记;不同种群间的遗传相似程度与其地理间距呈反比;种群内的遗传相似程度比种群间的高;利用UPGMA法可将其聚为冬麦区和春麦区两大类群。     

中国西部麦红吸浆虫(双翅目:瘿蚊科)酯酶同工酶与种群遗传结构研究(英文)

本文用PAGE方法测定了我国西部麦红吸浆虫Sitodiplosismosellana (G啨ｈｉｎ) 3个地理种群酯酶同工酶 ,分析了其遗传规律及种群的遗传结构。采样地点有春麦区的皋兰县 (36.3°N ,1 0 3.9°E)和武威市(37.9°N ,1 0 2 .6°E)及冬麦区的长安县 (34.1°N ,1 0 8.9°E)。结果分析认为该酶受两个基因位点控制 ,命名为Est 1和Est 2。Est 1可能为质体基因 ,其酶谱为所有带中移动最快的一条 ,每个个体都有。Est 2为重复基因位点 ,共观察到 8个等位基因 ,在所有种群中表现为 8条带 ,依其迁移速度命名为a、b、c、d、e、f、g、h。Est 2在每个个体中表现 1 - 4条带 ,且为一多态位点 ,因此该等位酶可作为一个稳定的遗传标记。在所有研究种群的个体中 ,共观察到 1 9种酶谱类型。在冬麦区长安种群中个体酶谱类型多达1 7个 ;春麦区个体酶谱类型少 ,在皋兰种群内有 5个、武威种群内有 4个。在所有的种群中 ,以d、e、g 3个等位基因的频率最高。冬麦区长安种群内有 8个等位基因、而春麦区种群仅有 3个。通过对Est 2单个基因位点的遗传一致度和聚类分析表明 ,春麦区两种群亲缘关系较近 ,且都与冬麦区种群较远。上述所有分析显示麦红吸浆虫有一定程度的种下分化 ,遗传漂移可能是引起该分化的主要原因。不同种群间有可能发生过     

用重复序列引物PCR分析不同滞育状态麦红吸浆虫DNA多态性

应用 5 个重复序列引物,通过 PCR 扩增试验,研究了不同滞育状态麦红吸浆虫 DNA 的多态性。结果表明:1) 5 个重复序列引物共扩增了 104 条核酸带,分子量介于 202~1 163bp 之间;2) 不同滞育状态的麦红吸浆虫的平均相似性指数范围在 0.573~0.936 之间,在种群 3 和种群 4 之间,最大的平均相似性指数是 0.936,在种群 1、3、4、5 和种群 6、7、8 之间平均相似性指数较高(均超过 0.81);3)不同滞育状态麦红吸浆虫群体的遗传变异大部分来自群体间,产生于群体间的变异为62.41%,来自群体内的变异为37.59%;4) 根据对不同滞育状态间遗传距离的聚类分析,麦红吸浆虫的滞育类型可分为三大类。首次报道了不同滞育状态麦红吸浆虫量化的DNA多态性。     

皱大球蚧(Eulecanium kuwanai)和瘤坚大球蚧(Eulecanium gigantean)地理种群的RAPD遗传分化

采用RAPD技术测定分析了河北省皱大球蚧和瘤坚大球蚧8个地理种群的遗传结构。结果表明：5种引物在8个种群中共产生了65条RAPD标记,各地理种群之间没有产生各自的特征标记;不同种群间的遗传相似程度与其地理间距呈反比;种群内的遗传相似程度比种间高。Shannon信息指数表明,皱大球蚧的平均遗传多样性高于瘤坚大球蚧,分别为0.3456和0.3225说明物种不同,其变异程度也不同。     

皱大球蚧(Eulecanium kuwanai)和瘤坚大球蚧(Eulecanium gigantean)地理种群的RAPD遗传分化

采用RAPD技术测定分析了河北省皱大球蚧和瘤坚大球蚧8个地理种群的遗传结构。结果表明：5种引物在8个种群中共产生了65条RAPD标记,各地理种群之间没有产生各自的特征标记;不同种群间的遗传相似程度与其地理间距呈反比;种群内的遗传相似程度比种间高。Shannon信息指数表明,皱大球蚧的平均遗传多样性高于瘤坚大球蚧,分别为0.3456和0.3225,说明物种不同,其变异程度也不同。     

应用RAPD技术分析奥利亚罗非鱼和尼罗罗非鱼的基因多态性

以随机扩增多态DNA技术(RAPD）分析了奥利亚罗非鱼和尼罗罗非鱼两个养殖群体的群体内及群体间遗传关系,并探讨了该技术在种群鉴定中的应用。RAPD引物筛选结果表明,所测试的20个随机引物中(Table 1),除一个引物未扩增出任何片段外,其余19个引物均扩增出1～11个大小不等的片段,长度大部分在500—3000bp之间,共扩增出220个片段,平均每个引物产生55个片段。两群体间共有片段70条,大部分引物的扩增产物具有种间多态性,种群间相似系数为0.727。以筛选的引物对两种群不同个体(Fig．1,Table 2)及种群混合样品(Fig.2,Table 3)进行RAPD分析。结果表明,不同引物在扩增图谱上表现很大差异：奥利亚罗非鱼不同个体间表现为一致的扩增图谱,种内相似系数达1000,显示了其种群内遗传变异的缺乏;尼罗罗非鱼种内相似系数为0．827,个体间存在不同程度的多态性;两个种群间的相似系数分别为0．767和0.742,表明种间有较高的同源性,遗传距离为0．235,略低于国外的报道．此外,两个养殖群体间的扩增图谱比较也暗示了遗传渐渗现象的存在。实验表明,RAPD标记可以作为一种可靠的遗传标记,用于不同鱼类种群的鉴定,RAPD分析方法是一种快速,简便且行之有鼓的鉴定鱼类种群的方法。     

中国麦红吸浆虫Sitodiplosis mosellana (Gehin)地理种群mtDNA COⅡ序列的遗传变异

对麦红吸浆虫Sitodiplosis mosellana(Gehin)11个地理种群线粒体DNA(mtDNA)细胞色素C氧化酶亚基Ⅱ(COⅡ)的部分片段进行了测序,分析了核苷酸的组成,构建了NJ分子系统树。结果表明,在用于分析的447bp序列中,A T平均含量为78．6％,其中7个位点存在变异。NJ树显示,麦红吸浆虫各种群间的亲缘关系与地理分布关系密切：11个地理种群可明显地聚为两大族群,所有来自春麦区的种群(NH、QX、GT、GW、GG)和冬麦区(陕西长安SC)种群聚为族群Ⅰ,其它冬麦区种群(HT、HL、HX、AS、AF)聚为族群Ⅱ;陕西长安种群(SC)虽处于冬麦区,但与春麦区种群具有很高的遗传相似性。该结果支持将我国麦红吸浆虫的发生区域分为三个,即春麦发生区、冬春麦发生区、冬麦发生区。各地理种群间的遗传距离为0～0．016,表现为种下的遗传变异,这与RAPD分析得出的结果相一致。     

山医群体中国地鼠近交E家系RAPD分析

目的　分析山医群体中国地鼠E家系的遗传纯度。方法　应用经过筛选的 3 1条随机引物对中国地鼠E家系 12只个体基因组DNA进行RAPD扩增 ,计算近交个体间的相似系数。结果　所有样品的相似系数0 943 1到 0 9978之间变动 ,平均相似系数为 0 9749,聚类分析得到了这些个体的同源树资料。结论　山医群体E家系有较高的遗传纯度     

麦红吸浆虫随气流远距离扩散的轨迹分析

为了解麦红吸浆虫Sitodiplosis mosellana (Géhin)种群随气流远距离扩散的可能性和扩散方向, 本研究于2010年5月在河南省洛阳市洛宁县, 利用系留气球携带取样器调查了麦红吸浆虫种群在5~75 m高空的分布以及活动节律, 应用HYSPLIT-4大气扩散模型模拟了2010年以洛宁县(34.35°N, 111.52°E)为起始点, 空中不同高度层麦红吸浆虫种群的扩散轨迹, 以及2007年麦红吸浆虫种群在我国北方麦区的扩散轨迹。结果表明: 在成虫发生期, 麦红吸浆虫在空中5, 45, 50和65 m 4个高度层种群密度较大, 表现出了明显的成层效应。2010年河南洛宁迁入的种群来自西南方的河南南阳地区, 迁出种群能够随气流进入东北方向的河南省宜阳县境内。2007年麦红吸浆虫种群能够随小麦发育期的先后, 随西南气流逐步向东北方向扩散。成虫随气流扩散是麦红吸浆虫种群远距离扩散的一种重要方式。研究结果有助于了解我国麦红吸浆虫远距离扩散方式, 同时对优化发生动态监测和综合治理提供参考。     

异源四倍体鲫鲤及其原始亲本遗传变异的微卫星标记分析

采用从鲤中分离出来的32对微卫星DNA标记,对异源四倍体鲫鲤、红鲫和野鲤的基因组DNA进行了研究。在筛选出的15对微卫星引物中,随引物不同,各等位基因数为1～8个,大小在100～420bp之间。从3个不同群体内部的遗传相似系数来看,异源四倍体鲫鲤个体之间的遗传相似系数最大,说明异源四倍体鲫鲤群体内部的遗传变异程度最低,已经形成了一个遗传性状稳定的群体。从3个不同群体之间的遗传相似系数来看,异源四倍体鲫鲤和红鲫遗传相似系数为0．5625,和野鲤的遗传相似系数为0．5125,说明异源四倍体鲫鲤接受原始母本的遗传物质比原始父本野鲤要多一些。微卫星标记与以前报道的RAPD标记的检测结果是相似的,然而由微卫星标记获得的种群内和种群间的遗传距离均大于RAPD,说明微卫星标记比RAPD标记显示出更高的个体多态性。     

Collagen-like triple helix formation of synthetic (Pro-Pro-Gly)10 analogues: (4(S)-hydroxyprolyl-4(R)-hydroxyprolyl-Gly)10, (4(R)-hydroxyprolyl-4(R)-hydroxyprolyl-Gly)10 and (4(S)-fluoroprolyl-4(R)-fluoroprolyl-Gly)10.

For the rational design of a stable collagen triple helix according to the conventional rule that the pyrrolidine puckerings of Pro, 4-hydroxyproline (Hyp) and 4-fluoroproline (fPro) should be down at the X-position and up at the Y-position in the X-Y-Gly repeated sequence for enhancing the triple helix propensities of collagen model peptides, a series of peptides were prepared in which X- and Y-positions were altogether occupied by Hyp(R), Hyp(S), fPro(R) or fPro(S). Contrary to our presumption that inducing the X-Y residues to adopt a down-up conformation would result in an increase in the thermal stability of peptides, the triple helices of (Hyp(S)-Hyp(R)-Gly)(10) and (fPro(S)-fPro(R)-Gly)(10) were less stable than those of (Pro-Hyp(R)-Gly)(10) and (Pro-fPro(R)-Gly)(10), respectively. As reported by B?chinger's and Zagari's groups, (Hyp(R)-Hyp(R)-Gly)(10) which could have an up-up conformation unfavorable for the triple helix, formed a triple helix that has a high thermal stability close to that of (Pro-Hyp(R)-Gly)(10). These results clearly show that the empirical rule based on the conformational preference of pyrrolidine ring at each of X and Y residues should not be regarded as still valid, at least for predicting the stability of collagen models in which both X and Y residues have electronegative groups at the 4-position.     

Synthesis and luminescence properties of a blue-emitting Sr(3.5) Y(6.5) O(2) (PO(4) )(1.5) (SiO(4) )(4.5) :Eu(2+) phosphor

A novel blue‐emitting Sr_3.5Y_6.5O₂(PO₄)_1.5(SiO₄)_4.5:Eu²⁺ phosphor was synthesized via a solid‐state reaction. Powder X‐ray diffraction (XRD) analysis demonstrated that the Sr_3.5Y_6.5O₂(PO₄)_1.5(SiO₄)_4.5 host had a hexagonal crystal structure in the space group P6₃/m and unit cell parameters a = 9.418 Å, c = 6.900 Å. The as‐prepared phosphor showed a blue emission and all the main emission peaks were located at around 466 nm for different excitation wavelengths of 297, 333 and 391 nm. The temperature dependence of the photoluminescence property was investigated in the range 20–250 °C, and the emission intensity decreased to 71% of the initial value at room temperature on increasing the temperature to 150 °C. According to the classical theory of fluorescent thermal quenching, the activation energy (ΔE) for the thermal quenching luminescence of the as‐prepared Sr_3.45Y_6.5O₂(PO₄)_1.5(SiO₄)_4.5:0.05Eu²⁺ phosphor was determined to be 0.20 eV. Copyright © 2011 John Wiley & Sons, Ltd.     

Role of tfdC(I)D(I)E(I)F(I) and tfdD(II)C(II)E(II)F(II) gene modules in catabolism of 3-chlorobenzoate by Ralstonia eutropha JMP134(pJP4)

The enzymes chlorocatechol-1,2-dioxygenase, chloromuconate cycloisomerase, dienelactone hydrolase, and maleylacetate reductase allow Ralstonia eutropha JMP134(pJP4) to degrade chlorocatechols formed during growth in 2,4-dichlorophenoxyacetate or 3-chlorobenzoate (3-CB). There are two gene modules located in plasmid pJP4, tfdC(I)D(I)E(I)F(I) (module I) and tfdD(II)C(II)E(II)F(II) (module II), putatively encoding these enzymes. To assess the role of both tfd modules in the degradation of chloroaromatics, each module was cloned into the medium-copy-number plasmid vector pBBR1MCS-2 under the control of the tfdR regulatory gene. These constructs were introduced into R. eutropha JMP222 (a JMP134 derivative lacking pJP4) and Pseudomonas putida KT2442, two strains able to transform 3-CB into chlorocatechols. Specific activities in cell extracts of chlorocatechol-1,2-dioxygenase (tfdC), chloromuconate cycloisomerase (tfdD), and dienelactone hydrolase (tfdE) were 2 to 50 times higher for microorganisms containing module I compared to those containing module II. In contrast, a significantly (50-fold) higher activity of maleylacetate reductase (tfdF) was observed in cell extracts of microorganisms containing module II compared to module I. The R. eutropha JMP222 derivative containing tfdR-tfdC(I)D(I)E(I)F(I) grew four times faster in liquid cultures with 3-CB as a sole carbon and energy source than in cultures containing tfdR-tfdD(II)C(II)E(II)F(II). In the case of P. putida KT2442, only the derivative containing module I was able to grow in liquid cultures of 3-CB. These results indicate that efficient degradation of 3-CB by R. eutropha JMP134(pJP4) requires the two tfd modules such that TfdCDE is likely supplied primarily by module I, while TfdF is likely supplied by module II.     

Induction of in vitro flowering in Dendrobium Madame Thong-In (Orchidaceae) seedlings is associated with increase in endogenous N(6)-(Delta (2)-isopentenyl)-adenine (iP) and N (6)-(Delta (2)-isopentenyl)-adenosine (iPA) levels

We analysed the endogenous cytokinin levels of Dendrobium Madame Thong-In seedlings grown in vitro during vegetative and flowering-inductive periods. HPLC was used to fractionate the extracts and radioimmunoassay (RIA) was used for assay of zeatin (Z), dihydrozeatin (DZ), N(6)-(Delta(2)-isopentenyl)-adenine (iP) and their derivatives. Coconut water used in experiments was found to contain high level (>136 pmol ml(-1)) of zeatin riboside (ZR). Protocorms and seedlings cultured in medium with coconut water were found to contain 0.5-3.9 pmol g(-1) FW of the cytokinins analysed. Seedlings (1.0-1.5 cm) cultured in flowering-inductive liquid medium containing 6-benzyladenine (BA, 4.4 muM) and coconut water (CW, 15%) contained up to 200 and 133 pmol g(-1) FW of iP and iPA, respectively. These levels were significantly higher than all other cytokinins analysed in seedlings of the same stage and were about 80- to 150-folds higher than seedlings cultured in non-inductive medium. During the transitional (vegetative to reproductive) stage, the endogenous levels of iP (178 pmol g(-1) FW) and iPA (63 pmol g(-1) FW) were also significantly higher than cytokinins in the zeatine (Z) and dihydrozeatin (DZ) families in the same seedlings. Seedlings that grew on inductive medium but remained vegetative contained lower levels of iPA. The importance of the profiles of iP and its derivatives in induction of in vitro flowering of D. Madame Thong-In is discussed.     

Biology of Bactrocera (Zeugodacus) tau (Walker) (Diptera: Tephritidae)

The biology of the fruit fly Bactrocera tau, an important horticultural pest, was studied under laboratory conditions at 25°C and 60–70% relative humidity on Cucurbita maxima. The duration of mating averaged 408.03 ± 235.93 min. After mating, the female fly had a preoviposition period of 11.7 ± 4.49 days. The oviposition rate was 9.9 ± 8.50 eggs and fecundity was 464.6 ± 67.98 eggs/female. Eggs were elliptical, smooth and shiny white, turning darker as hatching approached, and measured 1.30 ± 0.07 mm × 0.24 ± 0.04 mm. The chorion has polygonal microsculpturing and is species-specific with polygonal walls. The egg period lasts for 1.3 ± 0.41 days. The duration of the larval period is 1.2 ± 0.42, 1.7 ± 0.48 and 4.0 ± 0.94 days for first, second and third instars, respectively. Pupation occurs in the sand or soil and pupal periods are 7.0 ± 0.47 days. The life cycle from egg to adult was completed in 14.2 ± 1.69 days; the longevity of mated females and males was 130.33 ± 14.18 and 104.66 ± 31.21 days, respectively. At least two to three generations were observed from June 2008 to June 2009.     

Spectroscopic investigations of Er(3+) :CdO-Bi(2) O(3) -B(2) O(3) glasses

This article reports on the optical properties of Er³⁺ ions doped CdO–Bi₂O₃–B₂O₃ (CdBiB) glasses. The materials were characterized by optical absorption and emission spectra. By using Judd–Ofelt theory, the intensity parameters Ω_λ (λ = 2, 4, 6) and also oscillatory strengths were calculated from the absorption spectra. The results were used to compute the radiative properties of Er³⁺:CdBiB glasses. The concentration quenching and energy transfer from Yb³⁺–Er³⁺ were explained. The stimulated emission cross‐section, full width at half maximum (FWHM) and FWHM × values are also calculated for all the Er³⁺:CdBiB glasses. Copyright © 2011 John Wiley & Sons, Ltd.     

Cationic (tripyrrinato)palladium(II) complexes

The formation of cationic palladium(II)complexes [TrpyPd^II]⁺X⁻ by salt metathesis of the respective trifluoroacetates with different salts of weakly coordinating anions X⁻ was investigated. With non-hydrolizable counterions, cationic mono- and dinuclear complexes are observed depending on the nature of the anion X⁻ and the solvent. The mononuclear cations, which are only formed with X = BAr^F, most probably carry a weakly bound molecule of dichloromethane at the fourth coordination site of Pd^II. When treated with diazoalkanes, only these are sufficiently reactive to form carbene complexes. Four- and five coordinate Lewis base adducts [TrpyPd^IIL]⁺ with L = CH₃NC, tBuNH₂, PMe₃, PEt₃ and PiPr₃ and [TrpyPd^IIL₂]⁺ with L = PMe₃ were prepared from the mononuclear cations [TrpyPd^II]⁺BAr^F−. From structural studies it becomes apparent, that the formation of stable five coordinate Pd^II species is restricted to medium size ligands and depends on the delicate balance between the steric influence of L and the strain, which is induced on the TrpyPd^II unit.     

The helix-coil transitions of poly (dA)-poly (dT) and poly (dA-dT)-poly (dA-dT)

Helix–coil transition curves are calculated for poly (dA) poly(dT) and poly (dA-dT) poly (dA-dT) using the integral equation approach of Goel and Montroll.⁵ The transitions are described by the loop entropy model with the exponent of the loop entropy factor, k, remaining an arbitrary constant. The theoretical calculations are compared with experimental transition curves of the two polymers. Results indicate that the stacking energies for these two polymers differ by about 1 kcal/mole of base pairs. Also, a fit between theory and experiment was not possible for k > 1.70.