MASS ESTIMATE AND EVOLUTIONARY TREND IN CHINESE MESOZOIC FOSSIL BIRDS

体重是一项重要的生物学指标,生物的体重受到发育、繁殖和进化等诸多因素的影响.对于灭绝生物体重的估计有助于进一步恢复它们的各种生物学信息.本研究采用统计学的方法,对422件现生鸟类(分属于21目229种)的体重和18项骨骼量度指标分别进行一元回归分析,结果显示判定系数的分布范围在0.5 ～0.91之间,多数指标的判定系数均集中在0.8 ～0.9之间.采用另外64件测量有体重数据和骨骼量度的鸟样本对回归方程的估算准确率进行检验,发现前肢中肱骨长度和尺骨宽度以及后肢中胫跗骨宽度3项指标的估算准确率高于其他指标.分析结果还表明前肢两项指标对于估算鸣禽、猛禽和攀禽类等树栖鸟类的体重准确率较后肢显著;后肢指标对于估算陆禽类等地栖鸟类体重的准确率高于前肢指标.这一结果反映出与体重相关程度较高的骨骼量度指标在不同习性的鸟类当中存在着一定的差异.对于化石鸟类的体重估计,采用估算准确率较高并且便于测量的肱骨长度和胫跗骨宽度两项回归方程加以计算.通过对中国中生代鸟类的体重进行估算,结果显示中生代鸟类在系统发育过程中,反鸟类经历了体重逐渐减轻的过程,而今鸟类的体重开始不断增大并且出现显著的分异.     

Uncoupling protein-3 (UCP3) mRNA expression in reconstituted human muscle after myoblast transplantation in RAG2-/-/gamma c/C5(-) immunodeficient mice

Uncoupling protein-3 (UCP3), which is expressed abundantly in skeletal muscle, is one of the carrier proteins dissipating the transmitochondrial electrochemical gradient as heat and has therefore been implicated in the regulation of energy metabolism. Myoblasts or differentiated muscle cells in vitro expressed little if any UCP3, compared with the levels detected in biopsies of skeletal muscle. In the present report, we sought to investigate UCP3 mRNA expression in human muscle generated by myoblast transplantation in the skeletal muscle of an immunodeficient mouse model. Time course experiments demonstrated that 7-8 weeks following transplantation fully differentiated human muscle fibers were formed. The presence of differentiated human muscle fibers was assessed by quantitative PCR measurement of the human alpha-actin mRNA together with immunohistochemical staining using specific antibodies for spectrin and the slow adult myosin heavy chain. Interestingly, we found that the expression of UCP3 mRNA was dependant on human muscle differentiation and that the UCP3 mRNA level was comparable with that found in human muscle biopsies. Moreover, the human UCP3 (hUCP3) promoter seems to be fully functional, since triiodothyronine treatment of the mice not only stimulated the mouse UCP3 (mUCP3) mRNA expression but also strongly stimulated the hUCP3 mRNA expression in human fibers formed after myoblast transplantation. To our knowledge, this is the first time that primary myoblasts could be induced to express the UCP3 gene at a level comparable of that found in human muscle fibers.     

Fingerprinting of Mixed Bacterial Strains and BIOLOG Gram-Negative (GN) Substrate Communities by Enterobacterial Repetitive Intergenic Consensus Sequence-PCR (ERIC-PCR)

PCR-based genomic fingerprinting by use of enterobacterial repetitive intergenic consensus primers (ERIC-PCR) was evaluated for its use in fingerprinting DNA of mixed Gram-negative bacterial strains and BIOLOG Gram-negative (GN) microplate substrate communities. ERIC-PCR fingerprints of six different pure bacterial strains and a combined mixture of the strains were compared with fingerprints obtained by two more established methods: amplified ribosomal DNA restriction analysis (ARDRA) and random amplified polymorphic DNA analysis (RAPD-PCR). The ERIC-PCR fingerprint of the mixed strains was highly reproducible and was more species-specific and representative of the individual strain fingerprints than the ARDRA and RAPD-PCR fingerprints, respectively. ERIC-PCR fingerprinting of model and rhizosphere BIOLOG GN substrate communities also provided clearly distinguishable fingerprints. Results of this study suggest that ERIC-PCR represents a rapid and highly discriminating method for fingerprinting DNA of mixed Gram-negative bacterial strains and BIOLOG GN substrate communities. Received: 11 September 1998 / Accepted: 29 October 1998     

ArlR反应调节蛋白在表皮葡萄球菌不同生长期表达的检测

表皮葡萄球菌(Staphylococcus epidermidis,SE)是寄居在人体和黏膜表面的条件致病菌,因可在医疗植入材料表面形成生物膜(biofilm)而具有致病性。细菌双组分信号转导系统可调控生物膜形成,但其调控机制在SE中研究甚少。本课题对arlRS双组分信号转导系统的反应蛋白ArlR在细菌不同生长期的表达情况进行初步研究。首先构建ArlR原核表达质粒,用纯化重组ArlR免疫小鼠,获得多克隆抗-ArlR抗体,免疫Dot方法检测结果显示小鼠抗-ArlR血清效价>1∶100000。进一步采用蛋白免疫印迹法检测ArlR在SE1457野生株不同生长期中的表达水平,结果显示,ArlR在2h表达量较低,到4h达高峰,6～10h表达量较4h降低。利用反转录实时荧光定量聚合酶链反应检测arlR基因在不同生长期的转录水平,结果显示相应时间点ArlR蛋白表达水平与arlR基因转录水平一致。本研究结果为后期研究双组分信号转导系统arlRS对SE生物膜形成的影响奠定基础。     

Ion-pairing high-performance liquid chromatographic method for the detection of N-acetylaspartate and N-acetylglutamate in cerebral tissue extracts

An ion-pairing high-performance liquid chromatographic method for the determination of N-acetylaspartate and N-acetylglutamate using a C-18 column and a UV detection at 210 nm wavelength, by means of a diode array detector, is presented. A buffer containing 2.8 mM tetrabutylammonium hydroxide, 25 mM KH(2)PO(4), 1.25% methanol, pH 7. 00, is utilized for the isocratic separation of these N-acetylated amino acids, at a flow rate of 1 ml/min and a column temperature of 23 degrees C. The suitability of this chromatographic separation (without additional chromatographic steps prior to HPLC assay) to monitor variations both of N-acetylaspartate and of N-acetylglutamate in perchloric acid brain extracts from rats subjected to the impact acceleration model of diffuse brain injury is also reported. According to the data presented, this HPLC method allows the separation of the two N-acetylated amino acids considered from the many possible interfering compounds, commonly present in extracts of cerebral tissue, which have high extinction coefficients at 210 nm wavelength. Values of N-acetylaspartate and N-acetylglutamate determined by this method showed that cerebral trauma negatively affects both compounds, according to the severity of trauma itself.     

Characterization of humoral responses in mice immunized with plasmid DNAs encoding SARS-CoV spike gene fragments

The immunological characteristics of SARS-CoV spike protein were investigated by administering mice with plasmids encoding various S gene fragments. We showed that the secreting forms of S1, S2 subunits and the N-terminus of S1 subunit (residues 18-495) were capable of eliciting SARS-CoV specific antibodies and the region immediate to N-terminus of matured S1 protein contained an important immunogenic determinant for elicitation of SARS-CoV specific antibodies. In addition, mice immunized with plasmids encoding S1 fragment developed a Th1-mediated antibody isotype switching. Another interesting finding was that mouse antibodies elicited separately by plasmids encoding S1 and S2 subunits cooperatively neutralized SARS-CoV but neither the S1 nor S2 specific antibodies did, suggesting the possible role of both S1 and S2 subunits in host cell docking and entry. These results provide insights into understanding the immunological characteristics of spike protein and the development of subunit vaccines against SARS-CoV.