Tail Tip Proteins Related to Bacteriophage λ gpL Coordinate an Iron-Sulfur Cluster

Tail Tip Proteins Related to Bacteriophage λ gpL Coordinate an Iron-Sulfur Cluster

The assembly of long non-contractile phage tails begins with the formation of the tail tip complex (TTC). TTCs are multi-functional protein structures that mediate host cell adsorption and genome injection. The TTC of phage λ is assembled from multiple copies of eight different proteins, including g...

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Veröffentlicht in:Journal of molecular biology 2013-07, Vol.425 (14), p.2450-2462
Hauptverfasser: Tam, William, Pell, Lisa G., Bona, Diane, Tsai, Alex, Dai, Xiao Xian, Edwards, Aled M., Hendrix, Roger W., Maxwell, Karen L., Davidson, Alan R.
Format: Artikel
Sprache:eng
Schlagworte:
absorbance
adsorption
Amino Acid Sequence
Amino Acid Substitution
Bacteria
bacteriophage
Bacteriophage lambda - chemistry
Bacteriophage lambda - physiology
bacteriophages
Caudovirales
color
cysteine
Cysteine - metabolism
electron paramagnetic resonance spectroscopy
genome
Gram-negative bacteria
Gram-Negative Bacteria - virology
iron
Iron - metabolism
iron-sulfur cluster
Iron-Sulfur Proteins - chemistry
Iron-Sulfur Proteins - metabolism
Molecular Sequence Data
Mutant Proteins - chemistry
Mutant Proteins - metabolism
Oxygen - metabolism
Phage l
Phage N15
phage tail assembly
phage λ gpL
Protein Binding
proteins
Sequence Alignment
Spectrum Analysis
Sulfur - metabolism
Viral Tail Proteins - chemistry
Viral Tail Proteins - metabolism
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Zusammenfassung:The assembly of long non-contractile phage tails begins with the formation of the tail tip complex (TTC). TTCs are multi-functional protein structures that mediate host cell adsorption and genome injection. The TTC of phage λ is assembled from multiple copies of eight different proteins, including gpL. Purified preparations of gpL and several homologues all displayed a distinct reddish color, suggesting the binding of iron by these proteins. Further characterization of the gpL homologue from phage N15, which was most amenable to in vitro analyses, showed that it contains two domains. The C-terminal domain was demonstrated to coordinate an iron-sulfur cluster, providing the first example of a viral structural protein binding to this type of metal group. We characterized the iron-sulfur cluster using inductively coupled plasma-atomic emission spectroscopy, absorbance spectroscopy, and electron paramagnetic resonance spectroscopy and found that it is an oxygen-sensitive [4Fe-4S]2+ cluster. Four highly conserved cysteine residues were shown to be required for coordinating the iron-sulfur cluster, and substitution of any of these Cys residues with Ser or Ala within the context of λ gpL abolished biological activity. These data imply that the intact iron-sulfur cluster is required for function. The presence of four conserved Cys residues in the C-terminal regions of very diverse gpL homologues suggest that utilization of an iron-sulfur cluster is a widespread feature of non-contractile tailed phages that infect Gram-negative bacteria. In addition, this is the first example of a viral structural protein that binds an iron-sulfur cluster. [Display omitted] ► Phage tail tips are critical for assembly, host interaction, and DNA injection. ► Phage λ gpL is a conserved non-contractile tail tip protein. ► gpL coordinates an iron-sulfur cluster. ► Iron-sulfur cluster binding is a conserved feature of the gpL family. ► The iron-sulfur cluster is likely required for biological activity.
ISSN:0022-2836
1089-8638
DOI:10.1016/j.jmb.2013.03.032