Voula Kodoyianni scite author profile

We present the 4.8-Mb complete genome sequence of Salmonella enterica serovar Typhi strain Ty2, a human-specific pathogen causing typhoid fever. A comparison with the genome sequence of recently isolated S. enterica serovar Typhi strain CT18 showed that 29 of the 4,646 predicted genes in Ty2 are unique to this strain, while 84 genes are unique to CT18. Both genomes contain more than 200 pseudogenes; 9 of these genes in CT18 are intact in Ty2, while 11 intact CT18 genes are pseudogenes in Ty2. A half-genome interreplichore inversion in Ty2 relative to CT18 was confirmed. The two strains exhibit differences in prophages, insertion sequences, and island structures. While CT18 carries two plasmids, one conferring multiple drug resistance, Ty2 has no plasmids and is sensitive to antibiotics.

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Molecular basis of loss-of-function mutations in the glp-1 gene of Caenorhabditis elegans.

Kodoyianni

Maine

Kimble

1992

MBoC

142

126

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The glp-1 gene encodes a membrane protein required for inductive cell interactions during development of the nematode Caenorhabditis elegans. Here we report the molecular characterization of 15 loss-of-function (If) mutations of glp-1. Two nonsense mutations appear to eliminate glp-i activity; both truncate the glp-1 protein in its extracellular domain and have a strong loss-of-function phenotype. Twelve missense mutations and one in-frame deletion map to sites within the repeated motifs of the glp-1 protein (10 epidermal growth factor [EGF]-like and 3 LNG repeats extracellularly and 6 cdclO/SWI6, or ankyrin, repeats intracellularly). We find that all three types of repeated motifs are critical to glp-I function, and two individual EGF-like repeats may have distinct functions. Intriguingly, all four missense mutations in one phenotypic class map to the N-terminal EGF-like repeats and all six missense mutations in a second phenotypic class reside in the intracellular cdclO/ SWI6 repeats. These two clusters of mutations may identify functional domains within the glp-1 protein.

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Translational control of maternal glp-1 mRNA establishes an asymmetry in the C. elegans embryo

Evans

Crittenden

Kodoyianni

et al. 1994

Cell

225

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