2012
DOI: 10.1016/j.pep.2012.01.019
|View full text |Cite
|
Sign up to set email alerts
|

Folding and activity of mutant cystathionine β-synthase depends on the position and nature of the purification tag: Characterization of the R266K CBS mutant

Abstract: Cystathionine beta-synthase (CBS), a heme-containing PLP-dependent enzyme, catalyzes the condensation of serine and homocysteine to yield cystathionine. Missense mutations in CBS, the most common cause of homocystinuria, often result in misfolded proteins. Arginine 266, where the pathogenic missense mutation R266K was identified, appears to be involved in the communication between heme and the PLP-containing catalytic center. Here, we assessed the effect of a short affinity tag (6xHis) compared to a bulky fusi… Show more

Help me understand this report

Search citation statements

Order By: Relevance

Paper Sections

Select...
4

Citation Types

3
57
0
1

Year Published

2013
2013
2024
2024

Publication Types

Select...
7

Relationship

3
4

Authors

Journals

citations
Cited by 31 publications
(61 citation statements)
references
References 33 publications
3
57
0
1
Order By: Relevance
“…The corresponding mutagenesis oligonucleotides were as follows (capital letters designate the codon of the mutated residue): 5′-ccgcttcgacagtccgTCAtcccatgtgggtgtt (FWD E201S), 5′-aacacccacatgggaTGAcggactgtcgaagcgg (REV E201S), 5′-gaatgcccgcttcGTCagtccggaatccc (FWD D198V), 5′-gggattccggactGACgaagcgggcattc (REV D198V), 5′-cctgggtaacatgctgCTAtcctgctggcgggca (FWD S466L), and 5′-tgcccgccagcagggaTAGcagcatgttacccagg (REV S466L). Purification of recombinant proteins followed the protocols that we developed for various hCBS constructs carrying either cleavable GST at the N terminus or a permanent 6xHis tag at the C terminus with a few modifications (11,31,33). Protein concentration was determined by the Bradford method (Thermo Pierce) using BSA as a standard according to the manufacturer's recommendations.…”
Section: Methodsmentioning
confidence: 99%
See 2 more Smart Citations
“…The corresponding mutagenesis oligonucleotides were as follows (capital letters designate the codon of the mutated residue): 5′-ccgcttcgacagtccgTCAtcccatgtgggtgtt (FWD E201S), 5′-aacacccacatgggaTGAcggactgtcgaagcgg (REV E201S), 5′-gaatgcccgcttcGTCagtccggaatccc (FWD D198V), 5′-gggattccggactGACgaagcgggcattc (REV D198V), 5′-cctgggtaacatgctgCTAtcctgctggcgggca (FWD S466L), and 5′-tgcccgccagcagggaTAGcagcatgttacccagg (REV S466L). Purification of recombinant proteins followed the protocols that we developed for various hCBS constructs carrying either cleavable GST at the N terminus or a permanent 6xHis tag at the C terminus with a few modifications (11,31,33). Protein concentration was determined by the Bradford method (Thermo Pierce) using BSA as a standard according to the manufacturer's recommendations.…”
Section: Methodsmentioning
confidence: 99%
“…Protein concentration was determined by the Bradford method (Thermo Pierce) using BSA as a standard according to the manufacturer's recommendations. The CBS activity in the classical reaction was determined by a previously described radioisotope assay using [ 14 C(U)] L-serine as the labeled substrate, essentially as described elsewhere (11,33,34).…”
Section: Methodsmentioning
confidence: 99%
See 1 more Smart Citation
“…Preparation of the recombinant modified hCBSOPTΔ516-525, C-hCBSOPTΔ516-525, C-hCBSOPTΔ516-525 D444N, and C-hCBSOPTΔ1-39Δ516-525 D444N enzymes followed the protocols that we developed for various hCBS constructs either expressed with cleavable GST at their N terminus (37) or carrying a permanent 6xHis tag at their C terminus (38), with a few modifications (22). The deletions and the D444N pathogenic mutation were introduced by using a QuikChangeII XL mutagenesis kit (Agilent) according to the manufacturer's recommendations.…”
Section: Methodsmentioning
confidence: 99%
“…The deletions and the D444N pathogenic mutation were introduced by using a QuikChangeII XL mutagenesis kit (Agilent) according to the manufacturer's recommendations. Denaturing and native protein gel electrophoresis, Western blot, and the CBS activity assay in the absence and presence of AdoMet were performed essentially as described previously (37,38). The crystals were grown by the sitting and/or hanging-drop vapor-diffusion method at 293 K in 96-well and 24-well crystallization plates, respectively, according to the protocol described previously (22).…”
Section: Methodsmentioning
confidence: 99%