光学显微镜下细菌芽孢染色方法的探讨

由于细菌芽孢对水溶性染料具有较强的抗性,造成芽孢的染色较困难。加热、酸水解、机械摩擦等措施均可以提高芽孢的染色性能,对这些处理方法的优缺点进行分析,并对常规使用的Moeller法进行了改进,提出了一种更适合于微生物学实验课堂教学的细菌芽孢鉴别染色方法。     

Staining procedures for flow cytometric monitoring of bacterial populations

Dual or multiple parameter flow cytometric analysis is developing into a powerful method for characterizing microbial populations. The distinguishing of the populations only by assignment of size/shape measurements by scattered ligth renders as not satisfactory. To differentiate between the cells, the employment of a specific fluorescence marker is absolutely necessary. Methods are presented for the flow cytometric determination of DNA and the polymer poly-β-hydroxybutyrate (PHB) content in three different bacterial strains. The measurement of the 3β-hydroxysterol content enables the differentation between yeast and bacterial organisms in mixed microbial populations. Monitoring the ratio of live to dead bacterial cells in soil or water samples, e.g. in pure culture systems, is shown.     

Cytolethal distending toxin: a bacterial bullet targeted to nucleus

Cytolethal distending toxin (Cdt) is a newly added member of bacterial protein toxins that hijack the control system of eukaryotic cells. Cdts are produced by several pathogenic bacteria causing chronic infectious diseases. They are composed of three subunits, CdtA, CdtB and CdtC, which together form a ternary complex. CdtB is the active component, and CdtA and CdtC are involved in delivering the CdtB into the cells. The sophisticated strategy of Cdt to control host cells is CdtB-mediated limited DNA damage of the host cell chromosome, which triggers the response of the cell cycle checkpoint and results in G2 arrest in the cells. Cdt also induces apoptotic cell death of lymphocytes, which may be relevant to onset or persistence of chronic infection by the producing bacteria. The study of this toxin is expected to provide us information on a novel strategy by which bacteria interact with host cells.     

The History of Staining the Development of Cytological Staining

Perhaps no other period has contributed more to our knowledge of the cell than the period 1875-1895. During these years most fundamental cytological phenomena were seen and described. Mitosis, maturation and fertilization, the great cornerstones of cytology, were firmly laid by the remarkable researches of Flemming, Strasburger, Van Beneden, Oscar and Richard Hertwig, Boveri and many others. Upon these researches experimental cytology developed and the significance of the morphological phenomena to inheritance and development was pointed out by such masters as W. Roux, Weismann, O. Hertwig, Boveri and E. B. Wilson.     

The History of Staining the Development of Cytological Staining

Perhaps no other period has contributed more to our knowledge of the cell than the period 1875-1895. During these years most fundamental cytological phenomena were seen and described. Mitosis, maturation and fertilization, the great cornerstones of cytology, were firmly laid by the remarkable researches of Flemming, Strasburger, Van Beneden, Oscar and Richard Hertwig, Boveri and many others. Upon these researches experimental cytology developed and the significance of the morphological phenomena to inheritance and development was pointed out by such masters as W. Roux, Weismann, O. Hertwig, Boveri and E. B. Wilson.     

The History of Staining the Development of Bacteriological Staining Methods

The staining of bacteria is naturally of later origin than the use of dyes in histological work, as the systematic study of bacteria did not begin until after 1870. The use of dyes in this study followed very promptly after that date, however.     

Block-Surface Staining

A method is described by which the tissue exposed on sectioning a specimen embedded in paraffin can be visualized in situ. The fixed specimen is impregnated with lead acetate, dehydrated in dioxane, infiltrated with paraffin and embedded. Tissues exposed on sectioning are developed by applying to the cut surface of the block a solution of potassium sulphide in water. Concentrations of the reagents used and the time intervals for the procedure are dependent upon the size of the specimen and upon the degree of contrast required. The method is described as it was applied to the study of a small human fetus in cross section. Representative photographs are included to show the results obtained.