Improved Stability of the Jun-Fos Activator Protein-1 Coiled Coil Motif

Mason, Jody M.; Hagemann, Urs B.; Arndt, Katja M.

doi:10.1074/jbc.m701828200

Cited by 40 publications

(78 citation statements)

References 55 publications

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“…44 Recently, we investigated the kinetics of complex formation between cFos and JunW, JunW Ph1 , and the intermediate mutants (JunW Q21R , JunW E23K ) using stopped-flow analysis. 45 This study revealed that all of the possible peptide mixtures fold via a transiently populated dimeric intermediate. Of these, cFos-JunW E23K is the only dimer where the intermediate can be detected by equilibrium denaturation.…”

Section: Discussionmentioning

confidence: 97%

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Selectional and Mutational Scope of Peptides Sequestering the Jun–Fos Coiled-Coil Domain

Hagemann

Mason

Müller

et al. 2008

Journal of Molecular Biology

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Section: Discussionmentioning

confidence: 97%

“…1). 45 The probability of these two contrasting selection systems arriving at such similar sequences by chance is unfeasibly low, indicating that both systems indeed selected for similar properties. The sequence of helix JunW Ph2 differs from the sequences of JunW Ph1 and JunW especially in the hydrophobic core.…”

Section: Phage Selection and Analysismentioning

confidence: 97%

Selectional and Mutational Scope of Peptides Sequestering the Jun–Fos Coiled-Coil Domain

Hagemann

Mason

Müller

et al. 2008

Journal of Molecular Biology

Self Cite

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“…A further insight into the structural determinants of stability arose by dissecting the folding pathway of four c-Jun leucine zipper variants that bind with high affinity to c-Fos [24]. These encompassed a PCA-selected winner (JunW) [17], a phage-display-selected winner (JunW Ph1 ) [22] and two intermediate mutants.…”

Section: Folding Of Jun-fos Ap-1 Coiled-coil Motifsmentioning

confidence: 99%

iPEP: peptides designed and selected for interfering with protein interaction and function

Mason

Müller

Arndt

2008

Biochemical Society Transactions

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Semi-rational design is combined with PCAs (protein-fragment complementation assays) and phage-display screening techniques to generate a range of iPEPs (interfering peptides) that target therapeutically relevant proteins with much higher interaction stability than their native complexes. PCA selection has been improved to impose a competitive and negative design initiative on the library screen, thus simultaneously improving the specificity of assay 'winners'. The folding pathways of designed pairs imply that early events are dominated by hydrophobic collapse and helix formation, whereas later events account for the consolidation of more intricate intermolecular electrostatic interactions.

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“…Echoing an early suggestion that Fos and Jun leucine zipper domains be used as a molecular Velcro in biotechnology (53) are studies that utilized leucine zippers to verify the substrate for a tyrosine kinase (54), to facilitate the amyloid formation of ␣-synuclein (55), to enhance the interaction of different proteins in a yeast two-hybrid setup (56), and to help design synthetic leucine zipper peptides that exhibit extremely high affinity for heterodimerization (41,(57)(58)(59). This work presents a suite that incorporated Fos and Jun to solve different challenges faced in recombinant protein expression and purification.…”

Section: Discussionmentioning

confidence: 99%

Protein Interaction Module–assisted Function X (PIMAX) Approach to Producing Challenging Proteins Including Hyperphosphorylated Tau and Active CDK5/p25 Kinase Complex

Sui

et al. 2015

Molecular & Cellular Proteomics

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Many biomedically critical proteins are underrepresented in proteomics and biochemical studies because of the difficulty of their production in Escherichia coli. These proteins might possess posttranslational modifications vital to their functions, tend to misfold and be partitioned into bacterial inclusion bodies, or act only in a stoichiometric dimeric complex. Successful production of these proteins requires efficient interaction between these proteins and a specific "facilitator," such as a protein-modifying enzyme, a molecular chaperone, or a natural physical partner within the dimeric complex. Here we report the design and application of a protein interaction moduleassisted function X (PIMAX) system that effectively overcomes these hurdles. By fusing two proteins of interest to a pair of well-studied protein-protein interaction modules, we were able to potentiate the association of these two proteins, resulting in successful production of an enzymatically active cyclin-dependent kinase complex and hyperphosphorylated tau protein, which is intimately linked to Alzheimer disease. Furthermore, using tau isoforms quantitatively phosphorylated by GSK-3␤ and CDK5 kinases via PIMAX, we demonstrated the hyperphosphorylation-stimulated tau oligomerization in vitro, paving the way for new Alzheimer disease drug discoveries. Vectors for PIMAX can be easily modified to meet the needs of different applications. This approach thus provides a convenient and modular suite with broad implications for proteomics and biomedical research. Molecular & Cellular Proteomics

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Improved Stability of the Jun-Fos Activator Protein-1 Coiled Coil Motif

Cited by 40 publications

References 55 publications

Selectional and Mutational Scope of Peptides Sequestering the Jun–Fos Coiled-Coil Domain

Selectional and Mutational Scope of Peptides Sequestering the Jun–Fos Coiled-Coil Domain

iPEP: peptides designed and selected for interfering with protein interaction and function

Protein Interaction Module–assisted Function X (PIMAX) Approach to Producing Challenging Proteins Including Hyperphosphorylated Tau and Active CDK5/p25 Kinase Complex

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