2002-2016年华北平原植被生长状况及水文要素时空特征分析

基于MODIS增强型植被指数（EVI）资料,结合降水、GRACE重力卫星水储量（TWS）、地下水、土壤水等资料,分析华北平原植被2002-2016年间的生长状况及各水文要素时空分布特征。研究结果表明：（1）2002-2016年间华北平原植被呈好转趋势,降水、水储量、土壤水、地下水等水文要素值呈减少趋势。（2）黄淮平原区植被以农作物为主,植被覆盖度呈增加趋势,而降水、水储量、地下水、土壤水均呈减少趋势,超采地下水灌溉农作物是短期内保障粮食安全的重要措施。（3）燕山-太行山山麓平原区、冀鲁豫低洼平原区的城乡居民用地区域植被覆盖显著减少,而降水增多,水储量、土壤水、地下水减少,人类活动对植被和水文要素贡献量大。（4）山东丘陵农林区分布着林地和草地,这些区域生长季的植被指数呈减少趋势,与降水量减少呈正相关关系。在气候变化和人类活动影响的大背景下,探讨不同生态环境的植被生长特征,清楚植被对水文变化的响应机理,可以消除影响植被生长的不利因素,为制定合理用水制度提供理论依据。     

高温强光对温州蜜柑叶绿素荧光、D1蛋白和Deg1蛋白酶的影响及SA效应

以3年生温州蜜柑（Citrus unishiu Marc.）植株为试材,用叶绿素荧光分析、Western-blotting蛋白质印记技术及DAB（3,3'-二氨基联苯胺）显色法,研究了高温强光（38℃和1600 μmol?m-2?s-1）对叶片叶绿素荧光参数、PS（光系统）II反应中心D1蛋白和Deg1蛋白酶的影响和SA（水杨酸）的效应。结果表明,高温强光交互作用4 h后,叶片的初始荧光Fo升高,最大光能转化效率Fv/Fm、表观光合电子传递速率ETR及PSII的量子产额ΦPSII显著降低,在D1蛋白降解的同时,Deg1蛋白酶含量也下降,并伴有H2O2的积累。在高温强光下,外源的H2O2使叶绿素荧光动力学快相参数(Fi-Fo)/(Fp-Fo)值（反映PSII中QB非还原中心的数量）升高和I-P的斜率（反映PSII 活化中心还原态QA积累的值）下降,Fv/Fm、ETR、ΦPSII及D1蛋白和Deg1蛋白酶下降幅度增大;而外源的SA使这些参数下降幅度减小。这些结果说明,高温强光诱导H2O2的积累造成Deg1蛋白酶和光系统反应中心D1蛋白的降解,Deg1蛋白酶的减少也进一步限制了D1蛋白的周转,进而使温州蜜柑PSII反应中心遭到破坏,SA对光合机构光破坏有保护作用。     

NEK2 plays an active role in Tumorigenesis and Tumor Microenvironment in Non-Small Cell Lung Cancer

Abnormal expression and dysfunction of Never-in-mitosis-A-related kinase 2 (NEK2) result in tumorigenesis. High levels of NEK2 are related to malignant progression, drug resistance, and poor prognosis. However, the relationship between NEK2 levels and the occurrence of non-small cell lung cancer (NSCLC) remains unknown. This study aimed to explore the impacts of NEK2 on the oncogenesis of NSCLC and the tumor microenvironment. Downregulation of NEK2 inhibited A549 and H1299 cell proliferation, migration, and invasion, blocking cell cycle at the G0/G1 phase. Loss of NEK2 inhibited the release of IL-10 from tumor cells, M2-like polarization of macrophages, angiogenesis, and vascular endothelial cell migration. Furthermore, NEK2 deficiency inhibited tumor growth in vivo. Taken together, NEK2 knockdown inhibited the occurrence and development of NSCLC, M2 polarization of macrophages, and angiogenesis. The abnormal expression of NEK2 might not only indicate tumor progression and patient prognosis but also serve as a potential molecular therapeutic target with great development prospects.     

A newly discovered Bacteroides conjugative transposon,CTnGERM1, contains genes also found in gram-positive bacteria

Results of a recent study of antibiotic resistance genes in human colonic Bacteroides strains suggested that gene transfer events between members of this genus are fairly common. The identification of Bacteroides isolates that carried an erythromycin resistance gene, ermG, whose DNA sequence was 99% identical to that of an ermG gene found previously only in gram-positive bacteria raised the further possibility that conjugal elements were moving into Bacteroides species from other genera. Six of seven ermG-containing Bacteroides strains tested were able to transfer ermG by conjugation. One of these strains was chosen for further investigation. Results of pulsed-field gel electrophoresis experiments showed that the conjugal element carrying ermG in this strain is an integrated element about 75 kb in size. Thus, the element appears to be a conjugative transposon (CTn) and was designated CTnGERM1. CTnGERM1 proved to be unrelated to the predominant type of CTn found in Bacteroides isolates-CTns of the CTnERL/CTnDOT family-which sometimes carry another type of erm gene, ermF. A 19-kbp segment of DNA from CTnGERM1 was cloned and sequenced. A 10-kbp portion of this segment hybridized not only to DNA from all the ermG-containing strains but also to DNA from strains that did not carry ermG. Thus, CTnGERM1 seems to be part of a family of CTns, some of which have acquired ermG. The percentage of G+C content of the ermG region was significantly lower than that of the chromosome of Bacteroides species-an indication that CTnGERM1 may have entered Bacteroides strains from some other bacterial genus. A survey of strains isolated before 1970 and after 1990 suggests that the CTnGERM1 type of CTn entered Bacteroides species relatively recently. One of the genes located upstream of ermG encoded a protein that had 85% amino acid sequence identity with a macrolide efflux pump, MefA, from Streptococcus pyogenes. Our having found >90% sequence identity of two upstream genes, including mefA, and the remnants of two transposon-carried genes downstream of ermG with genes found previously only in gram-positive bacteria raises the possibility that gram-positive bacteria could have been the origin of CTnGERM1.     

Small scale genetic alterations contribute to increased mutability at the X-linked Hprt locus in vivo in Blm hypomorphic mice

BLM, the gene mutated in Bloom syndrome (BS), encodes an ATP-dependent RecQ DNA helicase that is involved in the resolution of Holliday junctions, in the suppression of crossovers and in the management of damaged replication forks. Cells from BS patients have a characteristically high level of sister chromatid exchanges (SCEs), and increased chromosomal aberrations. Fibroblasts and lymphocytes of BS patients also exhibit increased mutation frequency at the X-linked reporter gene HPRT, suggesting that BLM also plays a role in preventing small scale genomic rearrangements. However, the nature of such small scale alterations has not been well characterized. Here we report the characterization of Hprt mutations in vivo in Blm hypomorphic mice, Blm^tm1Ches/Blm^tm3Brd. We found that the frequency of Hprt mutants was increased about 6-fold in the Blm^tm1Ches/Blm^tm3Brd mice when compared to Blm^tm3Brd heterozygous mice or wildtype mice. Molecular characterization of Hprt gene in the mutant clones indicates that many of the mutations were caused by deletions that range from several base pairs to several thousand base pairs. While deletions in BLM-proficient somatic cells are often shown to be mediated by direct repeats, all three deletion junctions in Hprt of Blm^tm1Ches/Blm^tm3Brd mice were flanked by inverted repeats, suggesting that secondary structures formed during DNA replication, when resolved improperly, may lead to deletions. In addition, single base pair substitution and insertion/deletion were also detected in the mutant clones. Taken together, our results indicated that BLM function is important in preventing small scale genetic alterations. Thus, both large scale and small scale genetic alterations are elevated when BLM is reduced, which may contribute to loss of function of tumor suppressor genes and subsequent tumorigenesis.     

黄曲霉产木聚糖酶条件优化及酶解产物初步分析

一株能利用木糖及丰纤维素水解液产乙醇的黄曲霉Aspergillus flavus Z7具有产木聚糖酶的能力.通过单因素试验和正交试验优化了产酶培养基,得到最佳组分为玉米芯2%,尿素0.2%,酵母膏0.25%,K2HPO4 0.5%,NaNO,0.1%,MgSO4·7H2O 0.1%;单因素试验表明,用纱布代替塑料布密封摇瓶封口能显著提高产酶量;Z7在碱性条件下具有更强的产酶性能,在最优条件下发酵,能产生最大木聚糖酶活122.23IU/ml.通过薄层分析,验证了Z7产生的木聚糖酶具有水解木聚糖生成木糖及木寡糖的能力.     

Characterization of the putative tryptophan synthase β-subunit from Mycobacterium tuberculosis

The increasing emergence of drug-resistant tuberculosis （TB） poses a serious threat to the control of this disease. It is in urgent need to develop new TB drugs. Tryptophan biosynthetic pathway plays an important role in the growth and replication of Mycobacterium tuberculosis （Mtb）. The β-subunit of tryptophan synthase （TrpB） catalyzes the last step of the tryptophan biosynthetic pathway, and it might be a potential target for TB drug design. In this study, we overexpressed, purified, and characterized the putative TrpB-encoding gene Rv1612 in Mtb H37Rv. Results showed that Mtb His-TrpB optimal enzymatic activity is at pH 7.8 with 0.15 M Na^＋ or 0.18 M Mg^2＋ at 37℃. Structure analysis indicated that Mtb TrpB exhibited a typical β/α barrel structure. The amino acid residues believed to interact with the enzyme cofactor pyridoxal-5＇-phosphate were predicted by homology modeling and structure alignment. The role of these residues in catalytic activity of the Mtb His-TrpB was confirmed by site-directed mutagenesis. These results provided reassuring structural information for drug design based on TrpB.     

微生物法生产普鲁兰酶的研究

对产普鲁兰酶的出发菌株进行筛选和诱变,使酶活从22．10u／ml提高到了40．77u／ml,酶活提高了84．4％。随后对菌体产酶培养基进行了确定和优化,得到最佳发酵培养基,在此培养基下,菌体产酶达46．76u／ml,为原酶活的114．7％。     

Spread of North American wind-dispersed trees in future environments

Despite ample research, understanding plant spread and predicting their ability to track projected climate changes remain a formidable challenge to be confronted. We modelled the spread of North American wind-dispersed trees in current and future (c. 2060) conditions, accounting for variation in 10 key dispersal, demographic and environmental factors affecting population spread. Predicted spread rates vary substantially among 12 study species, primarily due to inter-specific variation in maturation age, fecundity and seed terminal velocity. Future spread is predicted to be faster if atmospheric CO(2) enrichment would increase fecundity and advance maturation, irrespective of the projected changes in mean surface windspeed. Yet, for only a few species, predicted wind-driven spread will match future climate changes, conditioned on seed abscission occurring only in strong winds and environmental conditions favouring high survival of the farthest-dispersed seeds. Because such conditions are unlikely, North American wind-dispersed trees are expected to lag behind the projected climate range shift.