Affiliation:
1. Laboratoire de Génétique Appliquée-URLGA,1 and
2. Laboratoire de Génétique Microbienne,2 Institut National de la Recherche Agronomique, Domaine de Vilvert, 78352 Jouy en Josas Cedex, France
Abstract
ABSTRACT
The identification of exported proteins by fusion studies, while well developed for gram-negative bacteria, is limited for gram-positive bacteria, in part due to drawbacks of available export reporters. In this work, we demonstrate the export specificity and use of the
Staphylococcus aureus
secreted nuclease (Nuc) as a reporter for gram-positive bacteria. Nuc devoid of its export signal (called Δ
SP
Nuc) was used to create two fusions whose locations could be differentiated. Nuclease activity was shown to require an extracellular location in
Lactococcus lactis
, thus demonstrating the suitability of Δ
SP
Nuc to report protein export. The shuttle vector pFUN was designed to construct Δ
SP
Nuc translational fusions whose expression signals are provided by inserted DNA. The capacity of Δ
SP
Nuc to reveal and identify exported proteins was tested by generating an
L. lactis
genomic library in pFUN and by screening for Nuc activity directly in
L. lactis
. All Δ
SP
Nuc fusions displaying a strong Nuc
+
phenotype contained a classical or a lipoprotein-type signal peptide or single or multiple transmembrane stretches. The function of some of the predicted signals was confirmed by cell fractionation studies. The fusions analyzed included long (up to 455-amino-acid) segments of the exported proteins, all previously unknown in
L. lactis
. Homology searches indicate that several of them may be implicated in different cell surface functions, such as nutrient uptake, peptidoglycan assembly, environmental sensing, and protein folding. Our results with
L. lactis
show that Δ
SP
Nuc is well suited to report both protein export and membrane protein topology.
Publisher
American Society for Microbiology
Subject
Molecular Biology,Microbiology
Cited by
96 articles.
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