C. E. Nwoguh scite author profile

A rapid and sensitive method for detection of cell- and compartment-specific gene expression in individual cells of both Gram-negative and Gram-positive microorganisms is described. The method combines the use of gene fusions to lacZ, and a fluorogenic beta-galactosidase substrate, fluorescein-di-(beta-D-galactopyranoside), with digitized video microscopy. All of the reporter constructs tested were successfully detected. Secondary staining of the cells with a nucleic acid-specific dye, propidium iodide, allowed cells devoid of nucleic acid to be identified, while cell nucleoid shape and the morphological stage of development could be correlated with the location of beta-galactosidase activity. The double-staining procedure was used to show that gene expression can be induced in non-culturable cells of Salmonella enteritidis produced by carbon/nitrogen starvation. The resolution was sufficient to distinguish between cells at different morphological stages of sporulation in Bacillus subtilis. This highly sensitive and rapid method may have many other applications in basic and applied microbiology.

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A comparative study of the numbers of bacteria present in enteral feeds prepared and administered in hospital and the home

Anderton¹,

Nwoguh²,

McKune³

et al. 1993

Journal of Hospital Infection

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Detection of induced β‐galactosidase activity in individual non‐culturable cells of pathogenic bacteria by quantitative cytological assay

Nwoguh

Harwood

Barer³

1995

Molecular Microbiology

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One Escherichia coli and two F' lac+ Salmonella strains were carbon and nitrogen stressed at 37 degrees C over 35 days in the presence or absence of chloramphenicol; the number, activity and culturability of cells in the resultant populations were studied. Active cells were enumerated by fluorescence microscopy after treatment with the lac inducer IPTG and cytological assay for beta-galactosidase. In all experiments, active and total cell counts remained within a three-fold range of each other and their initial values, while culturability fell by > 10(8)-fold and 10(3)-fold in chloramphenicol-treated and untreated preparations, respectively. Quantitative image analysis revealed different distributions of cell-specific fluorescence and indicated a progressive decline in the levels of induced enzyme activity in both E. coli and Salmonella enteritidis. It was concluded that the non-culturable cells studied retained inducible enzyme activity and that this activity did not result from a starvation-induced programme of gene expression. Whether or not such active but non-culturable cells are viable, they are clearly responsive and have the potential to influence their environment. The assay described can be applied to heterogeneous populations and environments and shows considerable potential for the study of gene expression at the single cell level.

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Re-use of enteral feeding tubes—a potential hazard to the patient? A study of the efficiency of a representative range of cleaning and disinfection procedures

Anderton

Nwoguh

1991

Journal of Hospital Infection

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C. E. Nwoguh

The viable but non-culturable hypothesis and medical bacteriology

Use of digitized video microscopy with a fluorogenic enzyme substrate to demonstrate cell‐ and compartment‐specific gene expression in Salmonella enteritidis and Bacillus subtilis

A comparative study of the numbers of bacteria present in enteral feeds prepared and administered in hospital and the home

Detection of induced β‐galactosidase activity in individual non‐culturable cells of pathogenic bacteria by quantitative cytological assay

Re-use of enteral feeding tubes—a potential hazard to the patient? A study of the efficiency of a representative range of cleaning and disinfection procedures

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