Differential Interactions of Fluorescent Agonists and Antagonists with the Yeast G Protein Coupled Receptor Ste2p

Mathew, Elizabeth; Bajaj, Anshika; Connelly, Sara M.; Sargsyan, Hasmik; Ding, Fa‐Xiang; Hajduczok, Alexander; Naider, Fred; Dumont, Mark E.

doi:10.1016/j.jmb.2011.03.059

Cited by 23 publications

(49 citation statements)

References 46 publications

(92 reference statements)

Supporting

Mentioning

Contrasting

Order By: Relevance

“…16,17 Among the many synthetic β-turn peptidomimetics restricted by cyclization, (R)-γ-lactam conformational constraint incorporating [3-(R)-amino-2-oxo-1-pyrrolidineacetamido] in place of ProGly at residues 8 and 9 was reported to have the best activity only equal to that of parent peptide, [Nle ing approach involving the photoactivatable groups attached to the α-factor backbone was developed. 28,30,44,[51][52][53]55,56 pBenzoyl-L-phenylalanine (Bpa) and 3,4-Dihydroxyphenylalanine (DOPA) was reported to have a desirable property for this purpose, although incorporation of these groups at various positions in α-factor have been shown to result in a less than 30-fold decrease in receptor affinity. 44,51,55 Biotin (Bio) tagging modification of DOPA analog (Bio 7…”

Section: 16mentioning

confidence: 99%

“…40,41 On the other hand, those near the N-terminus of α-factor are responsible for triggering cell signaling through Ste2p or stabilizing the activated state of this receptor. 4,10,30,40,57 The two N-terminal Trp residues at position 1 and 3 are the key residues in the interaction between α-factor and the region of the receptor that promotes stimulation of the pheromone-responsive G protein pathway. 30,40,41 In addition, two N-terminal Trp residues preferentially insert into the cell membranes following interaction of α-factor with the phospholipid membrane.…”

Section: 39mentioning

confidence: 99%

“…4,10,30,40,57 The two N-terminal Trp residues at position 1 and 3 are the key residues in the interaction between α-factor and the region of the receptor that promotes stimulation of the pheromone-responsive G protein pathway. 30,40,41 In addition, two N-terminal Trp residues preferentially insert into the cell membranes following interaction of α-factor with the phospholipid membrane. 13,31 Based on the biological activity of lipopeptide conjugates and the combined role of the two Trp residues, 57 C-terminal extended analogs of α-factor with various number of Trp residues can be used to study highly potent α-factor analogs.…”

Section: 39mentioning

confidence: 99%

“…13,18,19,30,32 A study concerning cyclic α-factor analog mimicking β-turn structure in the center of α-factor provided additional proof that the constrained structure of the center of α-factor is deeply correlated with the potency of active analog. [18][19][20]30,32,43 These results show that the central β-turn near the receptor in the lipid membrane promotes interaction of the ligand with two sites in the receptor implicated in ligand binding (C-terminal region) and triggering of G protein signal transduction (Nterminal region). 4,30 Aib is sterically hindered by dialkylated side chains and thus its substitution generates a collapsed turn structure effectively.…”

Section: 1042mentioning

confidence: 99%

“…]α-factor) and 7-Nitrobenz-2-oxa-1,3-diazol-4-yl (NBD) 30,53,54 developed for the detection of ligand-receptor conjugates were shown to reduce activity to about 33% that of parent α-factor. 44,56 Although the conjugation strategy of photoactivatable groups is not focused on enhancing potency, all of these analogs display receptor affinities varying from slightly better than that of α-factor to about 6-fold lower.…”

mentioning

confidence: 99%

See 4 more Smart Citations

Highly Active Analogs of α-Factor and Their Activities Against Saccharomyces cerevisiae

Ahn¹,

Hong²,

Jin³

et al. 2014

Bulletin of the Korean Chemical Society

View full text Add to dashboard Cite

Thirteen analogs of tridecapeptide α-factor (WHWLQLKPGQPMY) of Saccharomyces cerevisiae with C-or N-terminal Trp extension and isosteric replacement by Aib at position 8 and 11, Trp at position 13, D-Ala at position 9, and Orn and Glu at position 6 were synthesized and assayed for their biological activity. Receptor binding assay was carried out using our newly developed spectrophotometric method with detector peptide 14. C-or N-terminal extended analogs, α-factor-[Trp] n (n =1-5) 1-5 and [N-Trp] 1 -α-factor 6, were all less active than native α-factor and gradual decreases in both activity and receptor affinity were observed with greater Trp extension. Trp-substituted analog at position 13, [Trp 13 ]α-factor 7, exhibited about 2-fold reductions in both activity and receptor affinity. Aib-substituted analogs, [Aib 8 ]α-factor 8 and [Aib 11]α-factor 9, showed 5-to 10-fold reduction in activity as well as 3-fold reduction in receptor affinity compared to native α-factor. [Orn 6]α-factor 10 demonstrated strong potency with a 7.0-fold increase in halo activity as well as 1.8-fold increase in receptor affinity compared to native α-factor. ]α-factor 11 exhibited 15-fold higher halo activity as well as nearly 3-fold higher receptor affinity compared to native α-factor.

show abstract

Section: 16mentioning

confidence: 99%

Section: 39mentioning

confidence: 99%

Section: 39mentioning

confidence: 99%

Section: 1042mentioning

confidence: 99%

mentioning

confidence: 99%

See 3 more Smart Citations

Highly Active Analogs of α-Factor and Their Activities Against Saccharomyces cerevisiae

Ahn¹,

Hong²,

Jin³

et al. 2014

Bulletin of the Korean Chemical Society

View full text Add to dashboard Cite

show abstract

Invited review GPCR structural characterization: Using fragments as building blocks to determine a complete structure

et al. 2014

Self Cite

View full text Add to dashboard Cite

The structural characterization of G protein-coupled receptors has surged since the development of methodologies to facilitate the crystallization of these highly helical, seven transmembrane, integral membrane receptors. In the past seven years, eighteen GPCR structures were determined by X-ray crystallography. The crystal structures represent a static picture of these conformationally flexible signal transducers. Analyses that probe their dynamics and conformational changes require other techniques, in particular solution state nuclear magnetic resonance studies. Such investigations are challenged by the size of GPCRs, their α-helical structure, which limits resonance dispersion, their tendencies to aggregate in micellar preparations and their conformational heterogeneity. For many years, groups have been studying GPCR fragments as a means to overcome some of these difficulties. The results of these fragment analyses are presented here. Review of the literature reveals that much of the original work depended on circular dichroism, infra-red spectroscopy and fluorescence approaches. High resolution structures obtained by NMR are compared, where applicable, to the available crystal structures. In most cases, the work done on fragments by biophysical analysis is validated by these comparisons. Our perspective on the field of GPCR fragment analysis is presented together with the future goals that must be considered if work with fragments is continued.

show abstract

Spectrophotometric Determination of Affinities of α‐Factors for Their G Protein‐Coupled Receptors in Saccharomyces cerevisiae

Ahn

Kim

Jin

et al. 2015

Bulletin Korean Chem Soc

View full text Add to dashboard Cite

A new and relatively simple spectrophotometric technique has been developed for the accurate determination of α‐factor pheromone affinities for Ste2p whole cell receptor in yeast a‐cells. We designed and tested nine detector peptides containing mono‐ (ε412 = 14 500) or tri‐cysteine residues (ε412 = 43 660). The free unbound detector was detected using Ellman's reagent at 412 nm. Saturation binding studies using Saccharomyces cerevisiae Y 7925 ( MATa ) at a concentration of 2.5 × 1011 cells/mL with the highest affinity detector 1, [Orn6]α‐factor‐[Cys]3, resulted in a dissociation constant ( K D ) of 1.67 × 10−7 and total binding sites per cell (B cell = 29 500 sites/cell) comparable with those obtained using radiolabeled binding assays. Competitive binding assay using five nonchromogenic α‐factor analogs allowed for the determination of each K D value. [Orn6,d‐Ala9]α‐factor showed the highest receptor affinity ( K D = 1.03 × 10−7 M), which was threefold higher than that of native α‐factor. This assay provides rapid and convenient results for determining the relative affinities of nonchromogenic α‐factors and eliminates the need for radioactive waste disposal.

show abstract

Differential Interactions of Fluorescent Agonists and Antagonists with the Yeast G Protein Coupled Receptor Ste2p

Cited by 23 publications

References 46 publications

Highly Active Analogs of α-Factor and Their Activities Against Saccharomyces cerevisiae

Highly Active Analogs of α-Factor and Their Activities Against Saccharomyces cerevisiae

Invited review GPCR structural characterization: Using fragments as building blocks to determine a complete structure

Spectrophotometric Determination of Affinities of α‐Factors for Their G Protein‐Coupled Receptors in Saccharomyces cerevisiae

Contact Info

Product

Resources

About