基于B样条修匀公式的边缘检测的改进方法

边缘检测是图像分割中的一个重要部分．本文依据B样条修匀公式的图像边缘检测的基本思想，但又因为用B样条函数光滑后的图像对原始图像的逼近性并不十分精确，即它们的误差图像中残留着一些可能造成检测到的边缘线不连续或有用特征可能检测不到的边缘信息，为减少残量误差，本文对图像原型值采取盈亏修正，然后再对修正的图像使用B样条修匀公式做全息光滑曲面，重新得到的曲面改进了逼近性，同时还具有足够的光滑性和良好的保凸性．     

内联网络安全的研究与探讨

本文论述了当前内联网络网络安全工作对于国家安全和经济建设的重要意义、它所面临的种种威胁、网络安全体系功能需求，并阐述网络安全技术最新发展，给出了一个较为完备的安全体系可以采用的各种加强手段，包括防火墙、加密认证、网络安全扫描、入侵检测等技术。     

EPON上行方向物理编码子层的FPGA实现

目前EPON的物理层(其中包含物理编码子层)在上行方向尚无ASIC芯片可以直接使用，该文提出了EPON物理编码子层在上行方向的设计思想，并用FPGA实现，功能仿真的结果验证了该设计逻辑功能的正确性。     

牛泡沫病毒BFV3026 gag基因的克隆及其在大肠杆菌中的表达

从牛泡沫病毒BFV3026感染的胎牛肺细胞中提取Hirt DNA,PCR扩增BFV3026　gag基因。序列分析确证后，将其克隆于原核表达载体pET32A，重组质粒转化大肠杆菌BL21（DE3），经IPTG诱导，使Gag蛋白得以高效表达。SDS－PAGE及Western blot证实：表达蛋白占菌体总蛋白的40%，本工作的完成为Gag蛋白功能的研究奠定基础。     

松材线虫携带细菌的致病性

用松材线虫携带的3种细菌（菌株Njh,菌株Njt和菌株Njw)和2种线虫（松材线虫和拟松材线虫）为接种体，以黑松愈伤组织和黑松无菌苗为接种对象，分别用无菌线虫单独接种，细菌单独接种，细菌和无菌松材线虫混合接种，细菌和无菌的拟松材线虫混合接种等，测定对黑松愈伤组织和黑松无菌苗的致病能力，接种试验结果表明，单独用无菌松材线虫或松松材线虫接种，均不能使黑松愈伤组织褐变和无菌黑松苗枯萎，而用无菌线虫与上述3种细菌分别混合接种均能使黑松无菌苗发生枯萎及愈伤组织严重褐变，其中线虫和菌株Njh，线虫和菌株Njt致萎活性很强，线虫和菌株Njw致萎活性较弱，在自然界致病力弱的拟松材线虫与细菌混合接种同样能引起松苗严重萎蔫及愈伤组织褐变，实验室条件下，人工接种幼苗病害的发生与松材线虫携带的细菌密切相关，而与线虫的在关系不大，松材线虫所携带的细菌在这一病害过程中起至关重要的作用。     

基于PHP的校园公文发布系统的设计与实现

分析了校园公文发布系统的基本结构 ,给出该系统的设计思路 .在分析B/S结构和PHP技术特点的基础上 ,提出了校园公文发布系统的一种结构形式 ,并使用PHP MySQL技术实现了该系统的主要功能     

Identification of antiviral- relevant genes in the cultured fish cells induced by UV-inactivated virus

~~Identification of antiviral- relevant genes in the cultured fish cells induced by UV-inactivated virus~~     

新型中孔多金属氧酸盐复合材料光催化降解染料罗丹明B的研究

以胺修饰的中孔氧化硅为载体，通过自组装技术制备了一取代keggin结构的K5［Ni（H2O）PW11O39］(以下简称PW11Ni)复合材料，并研究了该复合材料对可溶性染料罗丹明B(简称RB)光催化的活性。实验结果表明。该复合材料光催化RB的活性高于RB的直接光解和PW11Ni均相光催化。其中，复合材料PW11Ni—APS—SiO2可在180min内使RB的转化率达到91．6％。具有一定的开发价值。     

N-terminal of L protein of vesicular stomatitis virus contains a new signal sequence

The L protein (241kD) of vesicular stomatitis virus (VSV) is the most important snbnnit of the replication complex. The existence of specific localization signal in the L protein was investigated by making recombinant constructs expressing truncated mutants of the L protein fused to green fluorescent protein (GFP) in transient transfection assays. The chimeric genes encoding varied N-terminal of L and GFP gene were put under the control of T7 promoter or CMV promoter. The fusion proteins were transiently expressed in BHK-21, COS-7, CHO or Hep G2 cells. When more than 120 residues were deleted or only 96 residues were kept on the N-terminal, the fusion proteins were shown to be distributed throughout the cells, cytoplasm and nucleus under the confocal microscope. However, other chimeric proteins with 120 or more amino acids were dotted and distributed in the perinuclear regions. And the fusion protein with 96—120 aa has the similar distribution. A thirteen-residue peptide QGYSFLHEVDKEA (108—120) was identified as localization signal, whose function would be absolutely distributed with the deficiency of D or V. Our results show that there is an independent localizing signal in N-terminal domain of L protein of VSV and this functional signal is conserved in different cell lines.     

Expression of human clotting factor Ⅸ mediated by recom- binant lentiviral vector in cultured cells and hemophilia B mice

To explore the expression of human clotting factor Ⅸ (hFⅨ) cDNA in vitro and the feasibility of gene therapy for hemophilia B mice mediated by recombinant lentiviral vector, a recombinant hFⅨ lentiviral vector driven by ubiquitin-C promoter, FUXW, and by ABP liver specific promoter, FAXW, was constructed respectively. Recombinant lentivirus was harvested from 293T cells by calcium phosphate-mediated transient cotransfection of three plasmids (transgene vector, CMV腞8.2, VSV-G). hFⅨ expression was detected in supernatant of 293T, BHK and L-02 cells infected with FUXW virus, whereas higher expression of hFⅨ levels (630 ng/106 cells/48 h) was detected only in L-02 cells infected with FAXW virus. Serum hFⅨ antigen was detected in all hemophilia B mice treated with FAXW virus by tail vein injection, an efficiency level of hFⅨ was observed (45 ng/mL, approximately 1% of normal human levels), the expression lasted for more than 60 d. The results indicated that HIV-based lentiviral vectors offer a promising approach to the gene therapy of hemophilia B.