沙门氏菌增菌培养基中细菌混合培养生长动力学的试验研究

本文就甘露醇亚硒酸盐和亚硒酸盐两种增菌培养基对沙门氏菌各血清变型的选择性增菌作用作了研究。研究述及37℃下沙门氏菌与埃希氏大肠杆菌、绿脓杆菌、普通变形杆菌三种竞争菌混合培养生长动力学过程,测出了评价增菌培养基优劣的客观指标EI值;按沙门氏菌传统分离方法,对加有终浓度为10~1、10~2、10~4、10~6、10~8个活菌/毫升的沙门氏菌株与正常人大便的两种增菌培养基,经37℃下孵育20至24小时后作SS琼脂平板划线分离和沙门氏菌血清学鉴定。通过两种培养基EI值及沙门氏菌分离结果的比较证实,甘露醇亚硒酸盐培养基对沙门氏菌株的选择性增菌作用明显优越于亚硒酸盐培养基(P<0.001)。     

PRELIMINARY STUDY ON INCREASING GROWTH AND REJUVENATION FOR OSSIFIED EELS WITH THE MICROECOLOGICS

This paper was adopting intestinal normal microbiota: Micrococcus tntestinalt, sp. and Beneckea campbell, and were prepared to microecologics, also gave a rebuild of intestinal micro ecospecies for ossified eels, and research effect of increasing growth and rejuvenation to them, by the microecologics. Moreover, specially to set up double-control, including a thyroideum medicament and an empty test group, for the comparison and analysis. Our results show that the intestinal microecologics of eel, for increasing growth and rejuvenation to ossified eels, that are botth achieve striking effect. But looked the thyroideum for increasing growth to ossified eels were be very effective. Nevertheless, which for rejuvenation was failed to take effect.Furthermore, we inc-lined to believe that the could be possible still significance of effect, if again added intestinal obligate anserobes of adult eels, and the cerebiogen into this microecologics.     

动物胃粘膜提取物对双歧杆菌的促生长作用

本文阐述了不同浓度的动物胃粘膜提取物对双歧杆菌生长繁殖的影响。试验结果表明,胃粘膜提取物对双歧杆菌有明显的促进作用,而且随着浓度增加为1％时,其菌数为4.45亿/ml,而不加提取物的菌数为2.53亿/ml,加胃粘膜提取物的比不加的菌数增长175.9％,促生长作用明显。证明胃粘膜提取物中含有促进双歧杆菌生长因子。     

A New Antiroll Device for Cryostat Wax Sectioning

A new antiroll device has been developed to replace the antiroll guide plate for cryostat wax sectioning. With this device, a continuous ribbon of 3-4 μm sections can be obtained. The sections are flat, uncreased. and compression is reduced to a minimum.     

Influence of a Small Number of Mature T Cells in Donor Bone Marrow Inocula on Reconstitution of Lymphoid Tissues and Negative Selection of a T Cell Repertoire in the Recipient

Allo-chimerism and clonal elimination of self antigen (Ag) (Ia + Mls-1^a) reactive Vβ6+ T cells were analyzed and compared between allogeneic bone marrow (BM) chimeras reconstituted with BM cells which had been treated with anti-Thy-1 monoclonal antibody (mAb) plus complement (C) (T^– chimeras) and BM chimeras which had been reconstituted with BM cells pretreated with anti-Thy-1 mAb alone (T⁺ chimeras). When lethally irradiated AKR (Mls-1^a) mice were reconstituted with BM cells from B10 or B10 H-2 congenic mice, both T⁺ and T^– chimeras were entirely free of signs of graft-versus-host reaction (GVHR). However, complete replacement of the AKR lymphoid tissues by donor BM cells was accomplished at an early stage in T⁺ chimeras but not in T^– chimeras. On the other hand, clonal elimination of Vβ6⁺ T cells reactive to the recipient Ag (Mls-1^a) was abolished in T⁺ chimeras but successfully induced in T^– chimeras. The Vβ6⁺ T cells not eliminated in T⁺ chimeras showed depressed responses against Mls-1^a antigens. The findings herein demonstrate that T cells which contaminate a BM inoculum survive in recipient mice after treatment with anti-Thy-1 mAb without C in vitro followed by BMT. The surviving T cells have been estimated to represent fewer than 0.5% of the BM cells inoculated. These cells appear to accelerate the full replacement of recipient lymphoid tissues by donor cells. Furthermore, the T cells which survive in the marrow inoculum influence eventually the development of a tolerant state in the T cell repertoire of the donor.     

Differentiation of Rickettsia japonica by Restriction Endonuclease Fragment Length Polymorphism Using Products of Polymerase Chain Reaction Amplification with Rickettsia rickettsii 190-Kilodalton Surface Antigen Gene Primers

Restriction fragment length polymorphism of polymerase chain reaction (PCR) amplification products differentiated Rickettsia japonica, a causative agent of Oriental spotted fever, from other spotted fever group (SFG) rickettsiae. Primer pair Rr190. 70p and Rr190. 602n of R. rickettsii 190-kDa antigen gene sequence primed genomic DNAs obtained from R. japonica, type strain YH and strains NT, NK, YKI, and TKN. The products were cleaved by PstI but not by AfaI restriction endonuclease. The PstI digestion pattern of PCR-products amplified from all strains of R. japonica was identical and easily differentiated from that of other SFG rickettsiae. The present study demonstrated a genotypic difference between R. japonica and other pathogenic SFG rickettsiae.