Improved PCR method for the creation of saturation mutagenesis libraries in directed evolution: application to difficult-to-amplify templates

Sanchis, Joaquı́n; Fernández, Layla; Carballeira, José Daniel; Drone, Jullien; Gumulya, Yosephine; Höbenreich, Horst; Kahakeaw, Daniel; Kille, Sabrina; Lohmer, Renate; Peyralans, Jérôme J.‐P.; Podtetenieff, John; Prasad, Shreenath; Soni, Prashant; Taglieber, Andreas; Wu, Sheng; Zilly, Felipe E.; Reetz, Manfred T.

doi:10.1007/s00253-008-1678-9

Cited by 126 publications

(110 citation statements)

References 42 publications

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“…For PEGylation experiments, the pTK-SM N100-GFP-V5 (WT) (1) was used to generate a cysteine-free mutant, SM N100 C31S,C46S (C-null) and C46S or C31S mutants (designated 31C and 46C, respectively). The C-null plasmid was used to generate single cysteine mutants with either T3C, T9C, T11C, G18C, S37C, V41C, S43C, S59C, G61C, L65C, S67C, S71C, S83C, or S87C mutations using megaprimer site-directed mutagenesis (11). The pCMV-Insig6xmyc (Insig-myc) (12) plasmid used for differential solubilization assays was a generous gift from Drs Michael S. Brown and Joseph L. Goldstein (University of Texas Southwestern, Dallas, TX).…”

Section: Methodsmentioning

confidence: 99%

The Regulatory Domain of Squalene Monooxygenase Contains a Re-entrant Loop and Senses Cholesterol via a Conformational Change

Howe

Chua

Stevenson

et al. 2015

Journal of Biological Chemistry

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Background: Squalene monooxygenase (SM), a rate-limiting cholesterol synthesis enzyme, is degraded in conditions of excess cholesterol. Results: The cholesterol-regulatory domain of SM is membrane-associated by a re-entrant loop and undergoes a cholesteroldependent conformational change. Conclusion: A cholesterol-induced conformational change appears to allow SM to be targeted for degradation. Significance: This is the first structural, mechanistic explanation for cholesterol-regulated SM degradation.

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Section: Methodsmentioning

confidence: 99%

The Regulatory Domain of Squalene Monooxygenase Contains a Re-entrant Loop and Senses Cholesterol via a Conformational Change

Howe

Chua

Stevenson

et al. 2015

Journal of Biological Chemistry

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“…We used megaprimer sitedirected mutagenesis (41) to mutate pTK-SM N100-GFP-V5 and pTK-SM-V5 to generate 49 alanine mutants as indicated in the figures. The pTK-SM N49-GFP-V5 construct was generated previously (8).…”

Section: Cholesterol-regulated Degron Of Squalene Monooxygenase Plasmmentioning

confidence: 99%

A conserved degron containing an amphipathic helix regulates the cholesterol-mediated turnover of human squalene monooxygenase, a rate-limiting enzyme in cholesterol synthesis

Chua

Howe

Jatana

et al. 2017

Journal of Biological Chemistry

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Edited by Dennis R. VoelkerCholesterol biosynthesis in the endoplasmic reticulum (ER) is tightly controlled by multiple mechanisms to regulate cellular cholesterol levels. Squalene monooxygenase (SM) is the second rate-limiting enzyme in cholesterol biosynthesis and is regulated both transcriptionally and post-translationally. SM undergoes cholesterol-dependent proteasomal degradation when cholesterol is in excess. The first 100 amino acids of SM (designated SM N100) are necessary for this degradative process and represent the shortest cholesterol-regulated degron identified to date. However, the fundamental intrinsic characteristics of this degron remain unknown. In this study, we performed a series of deletions, point mutations, and domain swaps to identify a 12-residue region (residues Gln-62-Leu-73), required for SM cholesterol-mediated turnover. Molecular dynamics and circular dichroism revealed an amphipathic helix within this 12-residue region. Moreover, 70% of the variation in cholesterol regulation was dependent on the hydrophobicity of this region. Of note, the earliest known Doa10 yeast degron, Deg1, also contains an amphipathic helix and exhibits 42% amino acid similarity with SM N100. Mutating SM residues Phe-35/Ser-37/Leu-65/Ile-69 into alanine, based on the key residues in Deg1, blunted SM cholesterol-mediated turnover. Taken together, our results support a model whereby the amphipathic helix in SM N100 attaches reversibly to the ER membrane depending on cholesterol levels; with excess, the helix is ejected and unravels, exposing a hydrophobic patch, which then serves as a degradation signal. Our findings shed new light on the regulation of a key cholesterol synthesis enzyme, highlighting the conservation of critical degron features from yeast to humans.

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“…In the present study we applied a "short-cut" quality control as reported earlier. [28] The quality was checked by performing sequence analyses of pooled plasmids for each library prior to transformation into the expression strain (Experimental Section). The results of such an analysis are shown in Table 1.…”

Section: Generation Of Saturation Mutagenesis Librariesmentioning

confidence: 99%

Directed Evolution of an Enantioselective Enoate‐Reductase: Testing the Utility of Iterative Saturation Mutagenesis

et al. 2009

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Directed evolution utilizing iterative saturation mutagenesis (ISM) has been applied to the old yellow enzyme homologue YqjM in the quest to broaden its substrate scope, while controlling the enantioselectivity in the bioreduction of a set of substituted cyclopentenone and cyclohexenone derivatives. Guided by the known crystal structure of YqjM, 20 residues were selected as sites for saturation mutagenesis, a pooling strategy based on the method of Phizicky [M. R. Martzen, S. M. McCraith, S. L. Spinelli, F. M. Torres, S. Fields, E. J. Grayhack, E. M. Phizicky, Science 1999, 286, 1153-1155] being used in the GC screening process. The genes of some of the hits were subsequently employed as templates for randomization experiments at the other putative hot spots. Both (R)-and (S)-selective variants were evolved using 3-methylcyclohexenone as the model substrate in the asymmetric bioreduction of the olefinic functionality, only small mutant libraries and thus minimal screening effort being necessary. Some of the best mutants also proved to be excellent catalysts when testing other prochiral substrates without resorting to additional mutagenesis/screening experiments. Thus, the results constitute an important step forward in generalizing the utility of ISM as an efficient method in laboratory evolution of enzymes as catalysts in organic chemistry.

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Improved PCR method for the creation of saturation mutagenesis libraries in directed evolution: application to difficult-to-amplify templates

Cited by 126 publications

References 42 publications

The Regulatory Domain of Squalene Monooxygenase Contains a Re-entrant Loop and Senses Cholesterol via a Conformational Change

The Regulatory Domain of Squalene Monooxygenase Contains a Re-entrant Loop and Senses Cholesterol via a Conformational Change

A conserved degron containing an amphipathic helix regulates the cholesterol-mediated turnover of human squalene monooxygenase, a rate-limiting enzyme in cholesterol synthesis

Directed Evolution of an Enantioselective Enoate‐Reductase: Testing the Utility of Iterative Saturation Mutagenesis

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