猴免疫缺陷病毒特异性免疫复合物沉着与猴AIDS多系统病变关系的探讨

目的观察猴免疫缺陷病毒(SIV)感染后,病毒特异性免疫复合物(IC)在不同时间、不同组织的沉着情况,初步研究其与AIDS多系统病变的联系。方法对8只不同时间感染SIV的恒河猴及1只未感染SIV的猴进行尸检以获取多系统组织标本,进行连续切片和IgG、C3、SIV p27免疫荧光染色,并对结果进行比较分析。结果IgG、C3、p27在多个猴、多种组织的相同位置出现相同模式的荧光表达,证明存在IC的沉着;其中脑血管周(8/8),心肌间微血管(6/8)、和淋巴结副皮质(6/8)及生发中心(5/8)是阳性率最高的部位,肾小球及肾间质、肠黏膜固有层也有较多IC的沉着,且在感染中、晚期IC出现的比例更高。结论SIV感染后出现广泛的SIV-IC沉积,且随病情的进展而加重;IC可能是SIV导致AIDS多系统病变的主要形式。针对此过程进行研究,可帮助了解AIDS并发多系统器官病变的机制及研究新的治疗方法。     

High-resolution mapping reveals linkage between genes in common bean cultivar Ouro Negro conferring resistance to the rust,anthracnose, and angular leaf spot diseases

Key message

Co-segregation analysis and high-throughput genotyping using SNP, SSR, and KASP markers demonstrated genetic linkage between Ur-14 and Co-3 ⁴ /Phg-3 loci conferring resistance to the rust, anthracnose and angular leaf spot diseases of common bean.

Abstract

Rust, anthracnose, and angular leaf spot are major diseases of common bean in the Americas and Africa. The cultivar Ouro Negro has the Ur-14 gene that confers broad spectrum resistance to rust and the gene cluster Co-3 ⁴ /Phg-3 containing two tightly linked genes conferring resistance to anthracnose and angular leaf spot, respectively. We used co-segregation analysis and high-throughput genotyping of 179 F_2:3 families from the Rudá (susceptible) × Ouro Negro (resistant) cross-phenotyped separately with races of the rust and anthracnose pathogens. The results confirmed that Ur-14 and Co-3 ⁴ /Phg-3 cluster in Ouro Negro conferred resistance to rust and anthracnose, respectively, and that Ur-14 and the Co-3 ⁴ /Phg-3 cluster were closely linked. Genotyping the F_2:3 families, first with 5398 SNPs on the Illumina BeadChip BARCBEAN6K_3 and with 15 SSR, and eight KASP markers, specifically designed for the candidate region containing Ur-14 and Co-3 ⁴ /Phg-3, permitted the creation of a high-resolution genetic linkage map which revealed that Ur-14 was positioned at 2.2 cM from Co-3 ⁴ /Phg-3 on the short arm of chromosome Pv04 of the common bean genome. Five flanking SSR markers were tightly linked at 0.1 and 0.2 cM from Ur-14, and two flanking KASP markers were tightly linked at 0.1 and 0.3 cM from Co-3 ⁴ /Phg-3. Many other SSR, SNP, and KASP markers were also linked to these genes. These markers will be useful for the development of common bean cultivars combining the important Ur-14 and Co-3 ⁴ /Phg-3 genes conferring resistance to three of the most destructive diseases of common bean.

     

Apelin-13 induces ERK1/2 but not p38 MAPK activation through coupling of the human apelin receptor to the Gi2 pathway

Apelin signaling to the family of mitogen-activated protein kinases (MAPKs), such as extracellular-regulated kinases 1/2 (ERK1/2) and p38 MAPK, through the coupling of apelin receptor (APJ) to G-protein, mediates important pathophysiological responses. Although apelin fragments have been reported to induce ERK1/2 activation through G_i-protein, the intracellular pathways by which APJ activates these MAPKs are only partially understood. Here, using stably transfected human embryonic kidney 293 (HEK293) cells overexpressing human APJ (HEK293-apelinR), we showed that apelin-13 signaling leads to ERK1/2 and p38 MAPK pathways through APJ activation. It was found in HEK293-apelinR cells that ERK1/2 activation was initiated by apelin-13 at 5 min, with the peak of activation occurring at 15 min, and a return to the basal level within 60 min. The activation of ERK1/2 appeared to be dose-dependent with a significant activation being observed at 10 nM apelin-13 and maximal activation at 100 nM. However, phosphorylated-p38 MAPK was not detected in HEK293-apelinR cells treated with apelin-13. We also shown that the apelin-13-induced ERK1/2 activation requires a coupling with pertussis toxin-sensitive G-protein, and that overexpression of dominant-negative G_i2 completely inhibits the apelin-13-induced ERK1/2 activation. In addition, treatment with apelin-13 resulted in a concentration-dependent reduction of forskolin-stimulated cAMP production. It is therefore suggested that apelin-13 activates ERK1/2 but not p38 MAPK, which involves the coupling of APJ to the G_i2 cascade. In conclusion, the ERK1/ 2, but not p38 MAPKpathway is activated by apelin-13 through coupling of human APJ to G_i2-protein, which contributes to cellular responses.     

Complete genome sequence of the bacterium Ketogulonicigenium vulgare Y25

Ketogulonicigenium vulgare is characterized by the efficient production of 2KGA from L-sorbose. Ketogulonicigenium vulgare Y25 is known as a 2-keto-L-gulonic acid-producing strain in the vitamin C industry. Here we report the finished, annotated genome sequence of Ketogulonicigenium vulgare Y25.     

Trigoxyphins H and I: two new daphnane diterpenoids from Trigonostemon xyphophylloides

Two new daphnane diterpenoids (1 and 2), together with four known analogues (3-6) were isolated from Trigonostemon xyphophylloides. Their structures were elucidated by spectroscopic analysis. Compounds 1 and 2 were evaluated for in vitro cytotoxic activities against the SPCA-1 (human lung cancer) and BEL-7402 (human hepatocellular carcinoma) cancer cell lines. Trigoxyphin I (2) showed modest cytotoxicity against two tumor cell lines.     

Design and application of highly responsive fluorescence resonance energy transfer biosensors for detection of sugar in living Saccharomyces cerevisiae cells

A protein sensor with a highly responsive fluorescence resonance energy transfer (FRET) signal for sensing sugars in living Saccharomyces cerevisiae cells was developed by combinatorial engineering of the domain linker and the binding protein moiety. Although FRET sensors based on microbial binding proteins have previously been created for visualizing various sugars in vivo, such sensors are limited due to a weak signal intensity and a narrow dynamic range. In the present study, the length and composition of the linker moiety of a FRET-based sensor consisting of CFP-linker(1)-maltose-binding protein-linker(2)-YFP were redesigned, which resulted in a 10-fold-higher signal intensity. Molecular modeling of the composite linker moieties, including the connecting peptide and terminal regions of the flanking proteins, suggested that an ordered helical structure was preferable for tighter coupling of the conformational change of the binding proteins to the FRET response. When the binding site residue Trp62 of the maltose-binding protein was diversified by saturation mutagenesis, the Leu mutant exhibited an increased binding constant (82 microM) accompanied by further improvement in the signal intensity. Finally, the maltose sensor with optimized linkers was redesigned to create a sugar sensor with a new specificity and a wide dynamic range. When the optimized maltose sensors were employed as in vivo sensors, highly responsive FRET images were generated from real-time analysis of maltose uptake of Saccharomyces cerevisiae (baker's yeast).     

Rht10基因对‘鲁麦15’农艺性状和光合生理特性的影响

利用鲁麦15、Rht10鲁麦15、Ms2鲁麦15及Ms2+Rht10鲁麦15近等基因系为试验材料,研究了Rht10基因对小麦农艺性状、净光合速率(Pn)、蒸腾速率(Tr)等光合生理特性的影响.结果表明,Rht10使小麦的挑旗、抽穗、开花期均推迟了4～5 d;Rht10对鲁麦15和Ms2鲁麦15的降秆强度分别为53.77%和53.00%,穗长显著缩短(P<0.05),千粒重显著减少,但对有效穂数无显著影响(P>0.05).含有Rht10基因的材料与不含此基因的材料之间的光合生理参数普遍存在显著差异,但在不同时期不同参数差异正负不同;在灌浆后期,Rht10对Pn有显著正效应(P<0.05);从开花期到灌浆后期,Pn与气孔导度(Gs)、胞间二氧化碳浓度(Ci)总体变化趋势相同,且相关性显著,表明Pn在一定程度上受气孔因素的限制;在灌浆中后期,Rht10对Gs有明显的正效应;在抽穗和开花期,Rht10对Tr有明显的正效应;Rht10对叶片水分利用效率(WUE)在4个生育期有明显的负效应.由此可见,Rht10基因对小麦的生育期、株高、穗长都有明显的不利影响,对各项光合生理参数也有普遍正向或负向的影响,在利用Rht10进行杂交育种时应充分考虑此基因带来的不利效应.