Pseudoenzymatic dealkylation of alkyltins by biological dithiols

We investigated the time dependence of the degradation of three alkyltin derivatives by a nine amino acid linear peptide (I₁LGCWCYLR₉) containing a CXC motif derived from the primary sequence of stannin, a membrane protein involved in alkyltin toxicity. We monitored the reaction kinetics using the intrinsic fluorescence of the tryptophan residue in position 5 of the peptide and found that all of the alkyltins analyzed are progressively degraded to dialkyl derivatives, following a pseudoenzymatic reaction mechanism. The end point of the reactions is the formation of a covalent complex between the disubstituted alkyltin and the peptide cysteines. These data agree with the speciation profiles proposed for polysubstituted alkyltins in the environment and reveal a possible biotic degradation pathway for these toxic compounds.     

Characterization of the Tn916 Conjugative Transposon in a Food-Borne Strain of Lactobacillus paracasei

Food-borne antibiotic-resistant lactic acid bacteria have received growing attention in the past few years. We have recently identified tetracycline-resistant Lactobacillus paracasei in samples of milk and natural whey starter cultures employed in the manufacturing process of a typical Italian fermented dairy product, Mozzarella di Bufala Campana. In the present study, we have characterized at the molecular level the genetic context of tetracycline resistance determinants in these natural strains, which we have identified as tet(M). This gene was present in 21 independent isolates, whose fingerprinting profiles were distributed into eight different repetitive extragenic palindromic groups by cluster analysis. We provide evidence that the gene is associated with the broad-host, conjugative transposon Tn916, which had never before been described to occur in L. paracasei. PCR analysis of four independent isolates by use of specifically designed primer pairs detected the presence of a circular intermediate form of the transposon, carrying a coupling sequence (GGCAAA) located between the two termini of Tn916. This novel coupling sequence conferred low conjugation frequency in mating experiments with the recipient strain JH2-2 of Enterococcus faecalis.Several genetic determinants conferring tetracycline resistance have been described to occur in gram-positive, nonpathogenic bacteria (2, 20). Among them, tet(M), encoding a ribosomal protection protein, is most commonly found in lactic acid bacteria (LAB). The issue of antibiotic resistance spreading among commensal bacteria has received great interest in recent years, and the presence of antibiotic-resistant species in the environment, including food products, has been extensively reported (reviewed in references 2 and 20). Conjugative transposons represent important vehicles for dissemination of antimicrobial resistance within gram-positive and gram-negative bacteria (23). These elements can move from the genome of a donor bacterium to that of a recipient by conjugation (6). Tn916, an 18-kb element containing the genetic determinant for tetracycline resistance, was the first conjugative transposon to be identified. It carries the tet(M) gene and has a broad host range, comprising both gram-positive and gram-negative bacteria (7). Along with the tetracycline resistance gene, Tn916 carries the genes responsible for its own excision (xis) and integration (int) as well as the mob genes, which mediate conjugal transfer (4). The transposition process starts with excision of the transposon, mediated by the Int and Xis proteins, leading to the formation of a nonreplicative circular intermediate which is transferred to the recipient and integrates into a new target site. Excision represents the rate-limiting step and occurs through reciprocal, site-specific recombination between the nonhomologous regions located at the two termini of the integrated transposon, known as coupling sequences, which are retained in the circular intermediate (17).Lactobacillus paracasei belongs to the microbial group of LAB and represents, along with the closely related species Lactobacillus casei, one of the most common bacterial species employed in the food industry. It is naturally present in raw milk and in dairy products, such as typical cheeses obtained by traditional manufacturing procedures in different Mediterranean countries (1, 11, 18, 26). Moreover, due to its probiotic functions, it is also employed as food additive (3, 5). Among its beneficial properties for human health, a recent study suggested that L. paracasei can be considered a potential enhancer of systemic immunity (22). However, only a few studies analyzed antibiotic resistance in L. paracasei (15, 19).In the past few years, our studies have focused on the identification of genes responsible for antibiotic resistance in LAB isolated from traditional dairy foods manufactured without employing commercial starter cultures. Fermentation in such products is therefore carried out by natural starters, mostly reflecting the microbiological composition of raw milk, which is affected in turn by the environment in which the animals live. Moreover, selective pressure exerted by technological steps along the manufacturing procedure often has a deep impact on bacterial composition in the final product. The widespread use and misuse of antibiotics have applied strong selective pressure in the environment, favoring survival and spread of antibiotic-resistant species. It is therefore of special relevance to identify antibiotic resistance determinants in food-borne bacteria, their persistence along the production line of specific products, and their capability of horizontal transfer to those species that can colonize the human gut.In the present study, we have characterized at the molecular level a group of tetracycline-resistant L. paracasei isolates, previously identified in raw milk and natural whey starter cultures employed in the manufacture of the Italian traditional cheese Mozzarella di Bufala Campana (9). We provide evidence that in these isolates, tetracycline resistance is due to the presence of the conjugative transposon Tn916, carrying the tet(M) gene and capable of horizontal, interspecies transfer to the opportunistic pathogen Enterococcus faecalis via a circular intermediate containing a novel coupling sequence that confers a low-frequency-conjugation phenotype. Molecular analysis of the resulting primary E. faecalis transconjugants revealed the presence of a circular intermediate of Tn916 carrying the same coupling sequence found in the L. paracasei donor strains.     

Impaired assembly results in the accumulation of multiple HLA-C heavy chain folding intermediates

Class I MHC H chains assemble with beta2-microglobulin (beta2m) and are loaded with peptide Ags through multiple folding steps. When free of beta2m, human H chains react with Abs to linear epitopes, such as L31. Immunodepletion and coimmunoprecipitation experiments, performed in this study, detected a preferential association of L31-reactive, beta2m-free H chains with calnexin in beta2m-defective cells, and with calreticulin and TAP in beta2m-expressing cells. In beta2m-defective cells, the accumulation of calnexin-bound H chains stoichiometrically exceeded their overall accumulation, a finding that supports both chaperoning preferences and distinct sorting abilities for different class I folds. No peptide species, in a mass range compatible with that of the classical class I ligands, could be detected by mass spectrometry of acidic eluates from L31-reactive HLA-Cw1 H chains. In vitro assembly experiments in TAP-defective T2 cells, and in cells expressing an intact Ag-processing machinery, demonstrated that L31 H chains are not only free of, but also unreceptive to, peptides. L31 and HC10, which bind nearly adjacent linear epitopes of the alpha1 domain alpha helix, reciprocally immunodepleted free HLA-C H chains, indicating the existence of a local un-/mis-folding involving the N-terminal end of the alpha1 domain alpha helix and peptide-anchoring residues of the class I H chain. Thus, unlike certain murine free H chains, L31-reactive H chains are not the immediate precursors of conformed class I molecules. A model inferring their precursor-product relationships with other known class I intermediates is presented.     

The novel skeletal muscle sarcoplasmic reticulum JP-45 protein. Molecular cloning,tissue distribution,developmental expression,and interaction with alpha 1.1 subunit of the voltage-gated calcium channel

JP-45 is a novel integral protein constituent of the skeletal muscle sarcoplasmic reticulum junctional face membrane. We identified its primary structure from a cDNA clone isolated from a mouse skeletal muscle cDNA library. Mouse skeletal muscle JP-45 displays over 86 and 50% identity with two hypothetical NCBI data base protein sequences from mouse tongue and human muscle, respectively. JP-45 is predicted to have a cytoplasmic domain, a single transmembrane segment followed by an intralumenal domain enriched in positively charged amino acids. Northern and Western blot analyses reveal that the protein is mainly expressed in skeletal muscle. The mRNA encoding JP-45 appears in 17-day-old mouse embryos; expression of the protein peaks during the second month of postnatal development and then decreases approximately 3-fold during aging. Double immunofluorescence of adult skeletal muscle fibers demonstrates that JP-45 co-localizes with the sarcoplasmic reticulum calcium release channel. Co-immunoprecipitation experiments with a monoclonal antibody against JP-45 show that JP-45 interacts with the alpha1.1 subunit voltage-gated calcium channel and calsequestrin. These results are consistent with the localization of JP-45 in the junctional sarcoplasmic reticulum and with its involvement in the molecular mechanism underlying skeletal muscle excitation-contraction coupling.     

Assembly and selective "in synthesis" labeling of quenched fluorogenic protease substrates

Because impaired cellular protease activities are linked to many diseases, such as cancer, inflammation, neurodegeneration, and infection, internally quenched fluorescent peptides have recently been developed as tools for analyzing the specificities of these enzymes. Here we report convenient and cost-effective approaches for the selective "in synthesis" assembly of such substrate peptides for protease assays. Fluorescein and Dabcyl groups were covalently and selectively attached during synthesis to epsilon-amino groups of internal lysines. Functionality was then tested by digestion with leucine aminopeptidase, chymotrypsin, and microsomal vesicles. All peptides proved to be appropriate substrates of the enzymes tested and of the endogenous peptidases in the microsomal vesicles. In summary, we describe an innovative and cheap method to develop completely functional quenched fluorescent peptides that are usable in specific detection of individual proteases, in particular aminopeptidases, in both in vitro and in vivo systems.     

Effect of the [CCTG]n repeat expansion on ZNF9 expression in myotonic dystrophy type II (DM2)

Myotonic dystrophy is caused by two different mutations: a (CTG)n expansion in 3' UTR region of the DMPK gene (DM1) and a (CCTG)n expansion in intron 1 of the ZNF9 gene (DM2). The most accredited mechanism for DM pathogenesis is an RNA gain-of-function. Other findings suggest a contributory role of DMPK-insufficiency in DM1. To address the issue of ZNF9 role in DM2, we have analyzed the effects of (CCTG)n expansion on ZNF9 expression in lymphoblastoid cell lines (n=4) from DM2 patients. We did not observe any significant alteration in ZNF9 mRNA and protein levels, as shown by QRT-PCR and Western blot analyses. Additional RT-PCR experiments demonstrated that ZNF9 pre-mRNA splicing pattern, which includes two isoforms, is unmodified in DM2 cells. Our results indicate that the (CCTG)n expansion in the ZNF9 intron does not appear to have a direct consequence on the expression of the gene itself.     

Augmentation of the affinity of HLA class I-binding peptides lacking primary anchor residues by manipulation of the secondary anchor residues

A direct binding assay has been used to investigate the effect of the secondary anchor residues on peptide binding to class I proteins of the major histocompatibility complex. Based on predictions from a previous chemometric approach, synthetic peptide analogues containing unnatural amino acids were synthesized and tested for B*2705 binding. Hydrophobic unnatural amino acids such as α-naphthyl- and cyclohexyl-alanine were found to be excellent substituents in the P3 secondary anchor position giving peptides with very high B*2705-binding affinity. The binding to B*2705 of peptides optimized for their secondary anchor residues, but lacking one of the P2 or P9 primary anchor residues was also investigated. Most such peptides did not bind, but one peptide, lacking the P2 Arg residue generally considered essential for binding to all B27 subtypes, was found to bind quite strongly. These findings demonstrate that peptide binding to class I proteins is due to a combination of all the anchor residues, which may be occupied also by unnatural amino acids–a necessary step towards the development of peptidic or non-peptidic antagonists for immunomodulation.