阿扎霉素B(Azalomycin B)研究进展

介绍阿扎霉素B的生物学来源,研究历史,主要理化性质和结构确定,同时阐述了阿扎霉素B的生物合成途径,构效关系,生物学特性和应用前景。     

B.B.Brodie(1907～1989)

B.B.Brodie博土,一个先驱药理学家和美国国家科学院院士,1989年2月28日逝世。生前是美国国立卫生研究院心脏研究所化学药理实验室的创始人和第一任主任。     

Bücherbesprechung (Book Reviews)

Abstract

A field experiment was conducted during 2002 – 2003 and 2003 – 2004 to study the impact of controlling the insect vector, Whitefly, of yellow mosaic virus on the performance of green gram grown under rainfed lowland rice fallow situation. Insecticide, Imidachloprid 12.5 kg a.i./ha, was applied at 15- and 30-days growth to four green gram varieties, direct-sown under residual soil moisture conditions after the harvest of kharif rice. Results showed crops under YMV-management achieved 65.67% more seed yield producing 11.68 q/ha, which was significantly higher than the crops under no YMV management (7.05 q ha^?1). Plants which had been treated with insecticide were found to be less affected (8.50%) by YMV compared to those which had no treatment (20.10%). Varieties PDM 54 and PDM 11 emerged as superior, producing significantly higher seed yields, 12.73 and 11.69 q/ha respectively; while Pusa vishal (8.21 q ha^?1) and Pusa 105 (7.85 q ha^?1) produced moderately compared with the local variety (6.31 q ha^?1). In addition, PDM 54 and PDM 11 showed relatively more resistance against YMV infestation recording 5.23% and 6.01% infected plants.     

Liver Kinase B1 Suppresses Lipopolysaccharide-induced Nuclear Factor κB (NF-κB) Activation in Macrophages

Liver kinase B1 (LKB1), a serine/threonine kinase, is a tumor suppressor and metabolic regulator. Recent data suggest that LKB1 is essential in regulating homeostasis of hematopoietic cells and immune responses. However, its role in macrophages and innate immune system remains unclear. Here we report that macrophage LKB1 inhibits pro-inflammatory signaling in response to LPS. LPS-induced pro-inflammatory cytokines and pro-inflammatory enzymes were monitored in bone marrow-derived macrophages isolated from myeloid cell-specific LKB1 knock out mice and their wild type littermate control mice. LPS induced higher levels of pro-inflammatory cytokines and pro-inflammatory enzymes in bone marrow-derived macrophages from LKB1 KO than those from wild type mice. Consistently, LPS induced higher levels of NF-κB activation in LKB1-deficient macrophages than those in wild type. Further, LPS stimulation significantly increased LKB1 phosphorylation at serine 428, which promoted its binding to IκB kinaseβ (IKKβ), resulting in the inhibition of NF-κB. Finally, LPS injection caused higher levels of cytokine release and more severe tissue injury in the lung tissues of LKB1 KO mice than in those of control mice. We conclude that LKB1 inhibits LPS-induced NF-κB activation in macrophages.     

B链C端去七肽(B24～B30)胰岛素的分子置换法

一个几近失活的胰岛素类似物———B链C端去七肽 (B2 4～B30 )胰岛素(DHPI)已被结晶 .该晶体属于空间群P2 ₁2 ₁2 ₁,晶胞的 1个独立区内包含有 2个DHPI分子 .应用分子置换法确定了DHPI分子在晶胞中的取向和位置 ,并在 0 .3nm分辨率水平上构建了结构模型 .研究结果表明 ,一个独立区内的 2个DHPI单体分子由一个非晶体学 2次轴联系着 ,该局部 2次轴近似平行于晶体学c轴 .这一特性直接影响了自身旋转函数对该局部对称轴取向的确定     

Thioredoxin-mediated Denitrosylation Regulates Cytokine-induced Nuclear Factor κB (NF-κB) Activation

S-nitrosylation of nuclear factor κB (NF-κB) on the p65 subunit of the p50/p65 heterodimer inhibits NF-κB DNA binding activity. We have recently shown that p65 is constitutively S-nitrosylated in the lung and that LPS-induced injury elicits a decrease in SNO-p65 levels concomitant with NF-κB activation in the respiratory epithelium and initiation of the inflammatory response. Here, we demonstrate that TNFα-mediated activation of NF-κB in the respiratory epithelium similarly induces p65 denitrosylation. This process is mediated by the denitrosylase thioredoxin (Trx), which becomes activated upon cytokine-induced degradation of thioredoxin-interacting protein (Txnip). Similarly, inhibition of Trx activity in the lung attenuates LPS-induced SNO-p65 denitrosylation, NF-κB activation, and airway inflammation, supporting a pathophysiological role for this mechanism in lung injury. These data thus link stimulus-coupled activation of NF-κB to a specific, protein-targeted denitrosylation mechanism and further highlight the importance of S-nitrosylation in the regulation of the immune response.     

恐龙遗址旅游指南(3)欧洲篇(中B)

第三站:英国西德纳姆镇(Sydenhm)水晶宫公园(Crystal Palace Park) 离开刘易斯镇,我们原路返回伦敦市,继续这次朝圣之旅.我们先到著名的伦敦桥南端的伦敦桥站火车站(London Bridge),这个车站于1836年12月开始运营,以连结东南郊的通勤及短程列车为主,因此车站的早晚高峰时间极为拥挤混杂.     

Palmitate-induced PTP1B expression is mediated by ceramide-JNK and nuclear factor κB (NF-κB) activation

Palmitate induces PTP1B expression in skeletal muscle cells. The purpose of this study was to investigate the mechanisms responsible for palmitate-induced PTP1B expression in mouse skeletal muscle cells. Three truncated fragments of PTP1B promoter were cloned into PGL3-basic vector and the promoter activity of PTP1B was assessed in C2C12 cells exposed to palmitate either in the presence or in the absence of several inhibitors to study the biochemical pathways involved. EMSA was performed to examine binding of NF-κB to NF-κB consensus sequence and PTP1B oligonucelotides in the cells treated with palmitate. Lentiviral PTP1B-shRNA was used to knockdown PTP1B in myotubes. The phosphorylation and protein levels of IRS-1 and Akt were detected by western blot. 0.5mM palmitate induced PTP1B promoter activity in fragment -1715/+59 by 50% (p<0.01). Palmitate increased NF-κB binding to both NF-κB consensus sequence and one NF-κB sequence (-920 to -935) in PTP1B promoter. Incubation of C2C12 cells with different concentrations of C2-ceramide enhanced PTP1B promoter activity dose-dependently. Inhibitors of de novo ceramide synthesis prevented palmitate-induced PTP1B promoter activity in myotubes. In addition, inhibitor of JNK pathway prevented ceramide-induced PTP1B promoter activity in myotubes. Knockdown of PTP1B also prevented ceramide-reduced IRS-1 and Akt phosphorylations in the myotubes. Exposure of the cells to PMA and calphostin C, an inhibitor of PKC, did not affect the activity of PTP1B promoter. Our data provide the evidence that the mechanism by which palmitate increased the expression of PTP1B seems to be through a mechanism involving the activation of ceramide-JNK and NF-κB pathways.     

产生霍乱毒素B亚单位(CT—B)工程菌的发酵条件

高效表达霍乱毒索B亚单位的工程菌MM2菌株．在玉米浆培养基中能高效合成B亚单位,观察了吸光度(OD)、pH及B亚单位产生的动态变化。玉米浆培养基不仅成本低、制备工艺简易,而且B亚单位产量高,在50L发酵罐中培养,B亚单位产量可达40μg／mL。     

Studies on the genetic polymorphism of lactate dehydrogenase B (phenotype B−) in rodent erythrocytes

While the common red cell phenotype of lactate dehydrogenase in mammals includes A and B subunits, in some species, especially of the rodent suborder Myomorpha, LDH B subunits are absent in erythrocytes (phenotype B^–). A polymorphism involving LDH B⁺ and LDH B^– phenotypes was observed in Mus musculus, and it was found that LDH B^– is recessive in relation to LDH B⁺ (Shows and Ruddle, 1968). A similar polymorphism is described here in the field mouse, Apodemus sylvaticus. In family studies, the recessive mode of inheritance is confirmed. Induction of reticulocytosis reveals that the LDH B^– phenotype is not the consequence of degradation of the B subunits in aging red cells. The nature of the mutation giving rise to this polymorphism is discussed.Supported by the Deutsche Forschungsgemeinschaft.     

Structure of desheptapeptide (B24–B30) insulin in a new crystal form

The structure of desheptapeptide (B24–B30) insulin (DHPI) in a new crystal form (form B) has been determined and refined to 0.2 nm resolution. The crystals were obtained under the same crystallization condition as previously reported crystal form (form A). The overall structures of the two crystal forms are similar but obvious differences can be observed in crystal packing and local conformation. The crystal structures of the two forms show that the two independent molecules in an asymmetric unit from a DHPI dimer, and the dimer formation buries more than 18.20 and 16.95 nm² of solvent accessible surfaces for form A and form B DHPI, respectively, the largest among insulin and insulin analogs ever reported. Close examination at crystal packing shows that the dimer-forming surface of DHPI, namely Surface II, is normally present in the association of insulin and insulin analogs in their crystal structures. The results demonstrate that Surface II is crucially important for the formation of two crystal forms under the same crystallization condition.     

B链N端去二肽(B1～2)C端去五肽(B26～30)胰岛素晶体结构的分子置换法研究

以B链羧端去五肽胰岛素(DPI)结构为模型,应用分子置换法对B链N端去二肽(B1～2)C端去五肽(B26～30)胰岛素(DesB1～2DPI)晶体结构进行了研究.DesB1～2DPI晶体单位晶胞中每个结晶学不对称单位包含1个DesB1～2DPI分子.交叉旋转函数和平移函数搜索均找到了明显突出的峰,确定了DesB1～2DPI分子在晶胞中的取向和位置.进一步的三维模型重建和结构精化结果巩固了DesB1～2DPI的分子置换法研究的正确性.     

Karyotyp und DNS-Gehalt von Bufo bufo,B. viridis,B. bufo × B. viridis und B. calamita (Amphibia,Anura)

The karyotypes in spermatogonial and leukocyte metaphases of the toads Bufo bufo, B. viridis and B. calamita (all 2n=22) were analysed and the DNA content of colchicine treated and Feulgen stained spermatogonial metaphase chromosomes measured microspectrophotometrically. The toad species possess similar karyotypes, but the chromosomes of B. bufo are somewhat longer than the chromosomes of B. viridis and B. calamita. All chromosomes of B. bufo contain significantly more than, but in no case twice as much DNA as their homologues in the other two species. Eight chromosomes of B. bufo contain 30–40%, three about 50% more DNA than their homologues in B. viridis. Exactly the same DNA-differences between both sets of chromosomes were found in B. bufo × B. viridis hybrids. Significant differences in the DNA amount of B. viridis and B. calamita exist only between the large chromosomes of these species. The ratio of the total DNA amount of the genomes in the three species is 1.49∶1.07∶1. These DNA-differences between the three toad species are confirmed by microspectrophotometric DNA measurements of their erythrocyte nuclei. It is supposed that these interspecific differences in DNA content of the toads are not a consequence of differential polyteny but are caused during the evolution process by local increase in DNA in all chromosomes of B. bufo and in the large chromosomes of B. viridis.     

Subunit structure and higher order assembly of the hemocyanins of the Melongenidae family: Melongena corona (Gmelin), Busycon canaliculatum (Linné), B. carica (Gmelin), B. contrarium (Conrad), and B. spiratum (Lamarck)

1. The hemocyanins of the Melongenidae family of marine gastropods: Melongena corona, Busycon canaliculatum, B. carica, B. contrarium, and B. spiratum exist in solution as multi-decameric aggregates characterized by sedimentation coefficients of approximately 105 S, 130 S, 150 S, 170 S, and higher values, corresponding to di-, tri-, tetra-, penta-, and larger multi-decameric particles. 2. The hemocyanins of B. contrarium and B. carica seem to form the largest decameric aggregates with the tri- to penta-decamers respresenting the major constitutents. Scanning transmission electron microscopy (STEM), both of unstained, freeze-dried and negatively-stained specimens, shows the presence of discrete aggregates consisting of up to ten decameric units. 3. The particle masses as determined by STEM mass measurements for individual molecules gave integral multiples of from 4.2 x 10(6) to 4.4 x 10(6) daltons ranging from about 8.2 x 10(6) daltons for the typical di-decamer of B. canaliculatum hemocyanin to as high as about 39 x 10(6) and 43 x 10(6) for the nano-and deca-decamers of B. contrarium hemocyanin. 4. The appearance of the higher multi-decamers in both negatively-stained and freeze-dried specimens suggest that they are formed by the addition of decameric units to a single di-decameric unit "tail-wise" in both directions. The higher aggregates formed seem to terminate with a closed head or collar at both ends of the assembly.