大肠杆菌F18菌株敏感和抵抗基因型仔猪十二指肠基因表达谱差异分析

文章运用Agilent 双标记表达谱芯片, 基于已建立的苏太猪大肠杆菌F18菌株敏感性和抗性型全同胞配对个体, 分析十二指肠组织基因表达谱差异, 旨在筛选导致仔猪断奶后腹泻和水肿病发生的大肠杆菌F18菌株受体相关基因, 探讨造成大肠杆菌病抗性和敏感性资源家系抗性差异的分子生物学机理。研究结果显示, 以Fold change绝对值大于2倍进行筛选, 在敏感型(GG基因型)对抗性型(AA基因型)配对组中, 差异基因共13个, 其中上调6个, 下调7个, 在以敏感型(AG基因型)对抗性型(AA基因型)配对组中, 共筛选出差异基因6个, 其中上调4个, 下调2个。经GO分析发现差异基因的生物学过程主要涉及免疫应答、胞外区修饰(如糖基化)、细胞黏附、信号转导等。通路发现大肠杆菌F18菌株抵抗性和敏感性差异基因主要涉及糖脂合成代谢以及炎症免疫相关通路, 经芯片筛选出的相关基因的功能还需进一步的研究验证。     

Notulae de Gesneriaceie Sinensibus (IX)

Ten new species, three new varieties and a new section of the family Gesneriaceae are described from China in the present paper. They are Tremacron urceolatum K. Y. Pan from Muli of SW Sichuan, T. obliquifolium K. Y. Pan from Miyi and Yanyuan of SW Sichuan, T. aurantiacum K. Y. Pan from Mabian and Pinshan of S Sichuan, lsometrum Sect. Chorianthera W. T. Wang et K. Y. Pan (with I. eximium Chun as the section type), Isometrum eximium Chun ex K. Y. Pan from Jiulong, Muli and Jinyang of SW Sichuan; Ancylostemon mairei (Levl.) Craib var. emeiensis K. Y. Pan from Mt. Emei of Sichuan, A. aureus (Franch.) Burtt var. angustifolius K. Y. Pan from Zhenkang of SW Yunnan, A. gamosepalus K. Y. Pan from Hanyuan, Yanyuan and Yuexi of SW Sichuan, A. rhombifolius K. Y. Pan from Meigu of SW Sichuan, A. ronganensis K. Y. Pan from Rong an of Guangxi; Corallodiscus flabellatus) (Craib) Burtt var. puberulus K.Y. Pan from Zhongdian and Deqin of NW Yunnan, Nanchuan of S Sichuan and Zayü of Xizang (Tibet), Beccarinda minima K. Y. Pan from Jinxiu and Xiangzhou of Guangxi, Boeica stolonifera K. Y. Pan from Fangcheng, Shiwandashan, Pingnan and Dongxing of S Guangxi, B. multinervia K. Y. Pan from Yingjiang of W Yunnan, and Paraboea barbatipes K. Y. Pan from Napo of W Guangxi and Xichou of SE Yunnan.     

Novel Reassortant Highly Pathogenic H5N2 Avian Influenza Viruses in Poultry in China

There has been multiple evidence that domestic poultry may act as a vessel for the generation of novel influenza A viruses. In this study, we have analyzed the evolution and pathogenicity of 4 H5N2 avian influenza viruses isolated from apparently healthy poultry from H5N1 virus endemic areas in China. Phylogenetic analysis revealed that two of these viruses, A/duck/Eastern China/1111/2011 (DK/EC/1111/11) and A/goose/Eastern China/1112/2011 (GS/EC/1112/11) were derived from reassortment events in which clade 2.3.4 highly pathogenic avian influenza (HPAI) H5N1 viruses acquired novel neuraminidase and nonstructural protein genes. Another two isolates, A/chicken/Hebei/1102/2010 (CK/HB/1102/10) and A/duck/Hebei/0908/2009 (DK/HB/0908/09), possess hemagglutinin (HA) gene belong to clade 7 H5 viruses and other genes from endemic H9N2 viruses, or from viruses of various subtypes of the natural gene pool. All of these H5N2 isolates bear characteristic sequences of HPAI virus at the cleavage site of HA, and animal experiments indicated that all of these viruses but DK/HB/0908/09 is highly pathogenic to chickens. In particular, DK/EC/1111/11 and GS/EC/1112/11 are also highly pathogenic to ducks and moderately pathogenic to mice. All of these 4 viruses were able to replicate in domestic ducks and mice without prior adaptation. The emergence of these novel H5N2 viruses adds more evidence for the active evolution of H5 viruses in Asia. The maintenance of the highly pathogenic phenotype of some of these viruses even after reassortment with a new NA subtypes, their ability to replicate and transmit in domestic poultry, and the pathogenicity in the mammalian mouse model, highlight the potential threat posed by these viruses to both veterinary and public health.     

Heterologous expression of Arabidopsis C-repeat binding factor 3 (AtCBF3) and cold-regulated 15A (AtCOR15A) enhanced chilling tolerance in transgenic eggplant (Solanum melongena L.)

Key message

Our study shows that the expression of AtCBF3 and AtCOR15A improved the chilling tolerance in transgenic eggplant.

Abstract

In an attempt to improve chilling tolerance of eggplant (Solanum melongena L) plants, Arabidopsis C-repeat binding factor 3 (AtCBF3) and cold-regulated 15A (AtCOR15A) genes both driven by an Arabidopsis RESPONSIVE TO DESSICATION 29A promoter (AtRD29A) were transferred into the plants of eggplant cultivar Sanyueqie. Two independent homozygous transgenic lines were tested for their cold tolerance. The leaves of the transgenic plants in both lines withered much slower and slighter than the wild-type plants after exposure to cold stress treatment at 2 ± 1 °C. The gene expression of AtCBF3 and AtCOR15A was significantly increased as well as the proline content and the levels of catalase and peroxidase activities, while the relative electrical conductivity and the malondialdehyde content were remarkably decreased in the transgenic plants compared with the wild type at 4 ± 0.5 °C. The results showed that the expression of the exogenous AtCBF3 and AtCOR15A could promote the cold adaptation process to protect eggplant plants from chilling stress.     

Leishmania mexicana pifanoi: in vivo and in vitro interactions between amastigotes and macrophages

Macrophages of the cell line J774 were used in a comparative study of virulence involving amastigote stages of Leishmania mexicana pifanoi isolated from macrophages (AMA-M) of the aforementioned cell line, amastigote forms grown in the UM-54-cell-free medium (AMA-C), and promastigote stages. The macrophage cultures were inoculated with AMA-M and AMA-C at the culture cell to parasite ratios of 1:3, 1:5, and 1:10. The macrophages were exposed to either kind of amastigotes for 24, 48, and 72 h. At the end of each of these periods, and for each dilution, the percentages of macrophages harboring the parasites within their cytoplasm and the mean numbers of intracellular parasite/macrophage were estimated on the basis of examination of 200 phagocytes. When either AMA-M or AMA-C were employed, after 24 h, the percentages of infected macrophages were, respectively, 84.5%, 89.0%, and 94.5% for the three aforementioned dilutions, the majority of the phagocytes containing 1-5 parasites. After 48- and 72-h exposures, the macrophages harbored 6-11 and 11-20 amastigotes/cell, respectively. Evidently intracellular multiplication of the amastigotes has taken place. In contrast to the results obtained with amastigote forms, after inoculations of the macrophages cultures with promastigotes at the dilutions previously used for amastigotes, only 48-78 phagocytes were found to contain intracellular stages within their cytoplasm. Many macrophages were parasite-free, especially when exposed to fewer promastigotes. Experiments in which 5 X10(6) promastigotes, AMA-M, or AMA-C were inoculated into the footpads of hamsters yielded the following results with regard to terminal footpad volumes: 1.57, 3.31, and 3.32 cm3, respectively. Evidently both kinds of amastigotes had equal virulence for hamsters; however, the promastigote stages were much les virulent for these experimental hosts.     

Selection of trkB-binding peptides from a phage-displayed random peptide library

Brain-derived neurotrophic factor (BDNF) shows potential in the treatment of neurodegenerative diseases, but the therapeutic application of BDNF has been greatly limited because it is too large in molecular size to permeate blood-brain barrier. To develop low-molecular-weight BDNF-like peptides, we selected a phage-displayed random peptide library using trkB expressed on NIH 3T3 cells as target in the study. With the strategy of peptide library incubation with NIH 3T3 cells and competitive elution with 1 μg/mL of BDNF in the last round of selection, the specific phages able to bind to the natural conformation of trkB and antagonize BDNF binding to trkB were enriched effectively. Five trkB-binding peptides were obtained, in which a core sequence of CRA/TXΦXXΦXXC (X represents the random amino acids, Φ represents T, L or I) was identified. The BDNF-like activity of these five peptides displayed on phages was not observed, though all of them antagonized the activity of BDNF in a dose-dependent manner. Similar results were obtained with the synthetic peptide of C1 clone, indicating that the 5 phage-derived peptides were trkB antagonists. These low-molecular-weight antagonists of trkB may be of potential application in the treatment of neuroblastoma and chronic pain. Meanwhile, the obtained core sequence also could be used as the base to construct the secondary phage-displayed peptide library for further development of small peptides mimicking BDNF activity.