六六六对大型溞生态学的影响

在实验室条件下,测定了六六六对大型溞(Daphnia magna Straus)存活、生长和生殖的影响。在25℃时,以心跳停止为死亡标准,六六六(以丙体计)对大型溞48小时LC50及其95%可信限为1.32±0.30ppm。以存活、生长和生殖为毒性标准,未觉察反应浓度(NOEC)为150ppb,最低觉察反应浓度(LOEC)为200ppb,其应用因子在0.11-0.15之间。内禀增长能力(rm)是更为敏感的指标,六六六浓度要降低至50ppb才无明显影响。       

母牛分枝杆菌制剂对T淋巴细胞增殖反应影响的研究

以氚标记胸腺嘧啶核苷(~3H-TdR)掺入法检测每分钟脉冲数(CPM),比较母牛分枝杆菌活菌悬液、辐射杀死菌悬液及高温杀死菌悬液对健康人外周血T淋巴细胞增殖反应的影响.以此作为评价治疗以细胞介导免疫为主的结核病免疫功能障碍免疫制剂效力的一个重要参数.在加入单一刺激因子实验中,对照组CPM为448±131;加入BCG、母牛分枝杆菌活菌悬液、辐射杀灭菌悬液以及高温杀死菌悬液的CPM分别为1037±194,2299±140,1819±528,994±186.这4种制剂的刺激指数均在2.0以上,尤其是母牛分枝杆菌活菌悬液、辐射杀死菌悬液分别为5.13,4.06.结果表明,母牛分枝杆菌3种制剂与BCG基本相似,在体外对T淋巴细胞增殖反应有明显的促进作用,其中以活菌悬液和辐射杀死菌悬液更为显著.另一试验中,以重组白细胞介素-2(rIL-2)作对照,BCG、母牛分枝杆菌悬液、辐射杀死菌悬液及高温杀死菌悬液分别加入rIL-2,目的在于观察菌体抗原加淋巴因子对T淋巴细胞增殖反应有无协同刺激作用.对照组的CPM为3721±1336,BCG加rIL-2组CPM为6904±1218;母牛分枝杆菌3种制剂的CPM分别为9544±172…     

Analysis of genetic diversity and population structure of peanut cultivars and breeding lines from China,India and the US using simple sequence repeat markers

Cultivated peanut is grown worldwide as richsource of oil and protein. A broad genetic base is needed for cultivar improvement. The objectives of this study were to develop highly informative simple sequence repeat(SSR)markers and to assess the genetic diversity and population structure of peanut cultivars and breeding lines from different breeding programs in China, India and the US. A total of 111 SSR markers were selected for this study, resulting in a total of 472 alleles. The mean values of gene diversity and polymorphic information content(PIC) were 0.480 and 0.429, respectively.Country-wise analysis revealed that alleles per locus in three countries were similar. The mean gene diversity in the US,China and India was 0.363, 0.489 and 0.47 with an average PIC of 0.323, 0.43 and 0.412, respectively. Genetic analysis using the STRUCTURE divided these peanut lines into two populations(P_1, P_2), which was consistent with the dendrogram based on genetic distance(G_1, G_2) and the clustering of principal component analysis. The groupings were related to peanut market types and the geographic origin with a few admixtures. The results could be used by breeding programs to assess the genetic diversity of breeding materials to broaden the genetic base and for molecular genetics studies.     

Molecular cloning of NHE1 from winter flounder RBCs: activation by osmotic shrinkage,cAMP, and calyculin A

In this report, wedescribe the cloning, cellular localization, and functionalcharacteristics of Na⁺/H⁺ exchanger 1 (NHE1)from red blood cells of the winter flounder Pseudopleuronectesamericanus (paNHE1). The paNHE1 protein localizes primarily to themarginal band and exhibits a 74% similarity to the trout -NHE, and65% to the human NHE1 (hNHE1). Functionally, paNHE1 sharescharacteristics of both -NHE and hNHE1 in that it is activated bothby manipulations that increase cAMP and by cell shrinkage,respectively. In accordance, the paNHE1 protein exhibits both proteinkinase A consensus sites as in -NHE and a region of high homology tothat required for shrinkage-dependent activation of hNHE1. Aftershrinkage-dependent activation of paNHE1 and resulting activation of aCl/HCO exchanger, their paralleloperation results in net uptake of NaCl and osmotically obliged water.Activation of paNHE1 by cAMP is at least additive to that elicited byosmotic shrinkage, suggesting that these stimuli regulate paNHE1 bydistinct mechanisms. Finally, exposure to the serine/threoninephosphatase inhibitor calyculin A potently activates paNHE1, and thisactivation is also additive to that induced by shrinkage or cAMP.

     

Slow rate during AF improves ventricular performance by reducing sensitivity to cycle length irregularity

Atrial fibrillation (AF) is characterized by short and irregular ventricular cycle lengths (VCL). While the beneficial effects of heart rate slowing (i.e., the prolongation of VCL) in AF are well recognized, little is known about the impact of irregularity. In 10 anesthetized dogs, R-R intervals, left ventricular (LV) pressure, and aortic flow were collected for >500 beats during fast AF and when the average VCL was prolonged to 75%, 100%, and 125% of the intrinsic sinus cycle length by selective atrioventricular (AV) nodal vagal stimulation. We used the ratio of the preceding and prepreceding R-R intervals (RR(p)/RR(pp)) as an index of cycle length irregularity and assessed its effects on the maximum LV power, the minimum of the first derivative of LV pressure, and the time constant of relaxation by using nonlinear fitting with monoexponential functions. During prolongation of VCL, there was a pronounced decrease in curvature with the formation of a plateau, indicating a lesser dependence on RR(p)/RR(pp). We conclude that prolongation of the VCL during AF reduces the sensitivity of the LV performance parameters to irregularity.     

Transforming growth factor beta (TGFbeta ) signaling via differential activation of activin receptor-like kinases 2 and 5 during cardiac development. Role in regulating parasympathetic responsiveness

Little is known regarding factors that induce parasympathetic responsiveness during cardiac development. We demonstrated previously that in atrial cells cultured from chicks 14 days in ovo, transforming growth factor beta (TGFbeta) decreased parasympathetic inhibition of beat rate by the muscarinic agonist, carbamylcholine, by 5-fold and decreased expression of Galpha(i2). Here in atrial cells 5 days in ovo, TGFbeta increased carbamylcholine inhibition of beat rate 2.5-fold and increased expression of Galpha(i2). TGFbeta also stimulated Galpha(i2) mRNA expression and promoter activity at day 5 while inhibiting them at day 14 in ovo. Over the same time course expression of type I TGFbeta receptors, chick activin receptor-like kinase 2 and 5 increased with a 2.3-fold higher increase in activin receptor-like kinase 2. Constitutively active activin receptor-like kinase 2 inhibited Galpha(i2) promoter activity, whereas constitutively active activin receptor-like kinase 5 stimulated Galpha(i2) promoter activity independent of embryonic age. In 5-day atrial cells, TGFbeta stimulated the p3TP-lux reporter, which is downstream of activin receptor-like kinase 5 and had no effect on the activity of the pVent reporter, which is downstream of activin receptor-like kinase 2. In 14-day cells, TGFbeta stimulated both pVent and p3TP-lux. Thus TGFbeta exerts opposing effects on parasympathetic response and Galpha(i2) expression by activating different type I TGFbeta receptors at distinct stages during cardiac development.