Alcohol
Volume 30, Issue 3 , Pages 183-191, July 2003

Effects of ethanol on gut-associated lymphoid tissues in a model of bacterial translocation: a possible role of apoptosis

Department of Internal Medicine, Multidisciplinary Laboratory of the University Hospital Clementino Fraga Filho, Federal University of Rio de Janeiro (UFRJ), Brazil 21941-590

Received 30 October 2002; received in revised form 4 June 2003; accepted 4 June 2003.

Editor: T.R. Jerrells

Abstract 

Chronic ethanol intake has been shown to be associated with immune suppression and impairment of epithelial barrier function. We investigated the effects of ethanol on intestinal immunity and its relation to bacterial translocation (BT). Male Wistar rats were assigned to one of three groups and received respective diets for 28 days. The ethanol-fed group [(EG); n=11] received a liquid diet containing 5% [volume/volume (vol./vol.)] ethanol; a pair-fed group [(PFG); n=11] received an isocaloric diet without ethanol; and a third (control) group [(CG); n=11] received water and chow ad libitum. On experimental day 29, animals in the EG and the PFG underwent distal ileum ligature and small intestine inoculation of a tetracycline-resistant Escherichia coli strain (TcR E. coli R6), by means of gastric intubation, followed by duodenal ligature. One hour after inoculation, mesenteric lymph nodes, right lobe of liver, spleen, and left kidney were excised for bacterial studies. Sections of jejunum and colon were immunostained, with the use of antibodies against immunoglobulin (Ig) A, T cells, macrophages, and proliferating cell nuclear antigen (PCNA). Apoptosis was determined by the terminal deoxynucleotidyltransferase TdT-mediated dUDP-biotin nick end labeling (TUNEL) method. Bacterial translocation rates were greater in the PFG compared with findings for the EG. Lamina propria of the jejunum of the EG showed a reduction in the densities of IgA+ cells and T cells compared with findings for the PFG and the CG. Colonic lamina propria of the EG showed reduced densities of IgA+ cells and macrophages compared with findings for the PFG and the CG. Apoptotic index was increased in the EG compared with findings for the PFG and the CG, in both jejunum and colon. Proliferation index was not significantly different among groups. Results of the current study show that chronic ethanol ingestion led to a reduction of cellular and humoral components of the intestinal mucosa, possibly by cell loss as a result of ethanol-induced apoptosis. The reduced rates of BT observed after chronic ethanol intake seem to indicate that factors irrespective of immune function might be involved in BT inhibition.

Keywords:  Ethanol, Bacterial translocation, Mucosal immunity, Apoptosis, Cell proliferation

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 The term “chronic” ethanol (alcohol) consumption (intake, exposure) is used heterogeneously across the literature. Although every attempt has been made, in this article, to provide the defining criterion or criteria used by investigators cited, the reader is advised to retrieve the published articles of the cited works to obtain technical details of the experiment and, thus, determine what constitutes “chronic” in the respective study designs. In the current study, chronic is defined as 28 days.

PII: S0741-8329(03)00134-4

doi:10.1016/S0741-8329(03)00134-4

Alcohol
Volume 30, Issue 3 , Pages 183-191, July 2003

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