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Use of antisense RNA to confer bacteriophage resistance in dairy starter cultures
Authors:Jeong Hwan Kim  Sung Guk Kim  Dae Kyun Chung  Yeou-Cherng Bor  Carl A Batt
Institution:(1) Department of Food Science, Cornell University, 413 Stocking Hall, 14853 Ithaca, NY, USA;(2) Present address: Department of Medical Microbiology and Immunology, Stanford University, Stanford, CA, USA;(3) Present address: Section of Biochemistry, Molecular and Cellular, Cornell University, Ithaca, NY, USA
Abstract:Summary The strategy and implementation of a unique system for engineering bacteriophage resistant starter cultures ofLactococcus lactis employing antisense RNA is reviewed. As a necessary prerequisite for developing this system, we have cloned and sequenced a number of bacteriophage genes coding for minor and major structural proteins. In addition, we have also identified a series of genes whose function(s) is not known but their sequences appear to be conserved in a vast number of isolates. One of these latter sequences, designatedgp51C, codes for a 51-kDa protein which is extremely charged and shares some homology with yeast translation intiation factor. Resistance to a broad class of isometric bacteriophages has been achieved by expression of an antisense RNA targeted against, for example,gp51C. In the best case, expression of the antisensegp51C RNA results is a greater than 99% reduction in the total number of plaque forming units. Additional antisense RNA constructs directed against other bacteriophage genes, including the major capsid protein, also appear effective at inhibiting infection from 40–55% suggesting that this approach may prove useful for engineering a set of truly isogenic strains to be used in a starter culture rotation plan.
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