2016
DOI: 10.1002/pmic.201600209
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Detergents: Friends not foes for high‐performance membrane proteomics toward precision medicine

Abstract: Precision medicine, particularly therapeutics, emphasizes the atomic-precise, dynamic, and systems visualization of human membrane proteins and their endogenous modifiers. For years, bottom-up proteomics has grappled with removing and avoiding detergents, yet faltered at the therapeutic-pivotal membrane proteins, which have been tackled by classical approaches and are known for decades refractory to single-phase aqueous or organic denaturants. Hydrophobicity and aggregation commonly challenge tissue and cell l… Show more

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Cited by 10 publications
(14 citation statements)
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References 178 publications
(397 reference statements)
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“…According to our results, the highest number of proteins is solubilized with Laemmli sample buffer containing 4% SDS. SDS is known for powerfully solubilizing membrane proteins . For example, it solubilizes the myelin membrane more efficiently than CHAPS or Triton X‐100 …”
Section: Discussionmentioning
confidence: 99%
See 1 more Smart Citation
“…According to our results, the highest number of proteins is solubilized with Laemmli sample buffer containing 4% SDS. SDS is known for powerfully solubilizing membrane proteins . For example, it solubilizes the myelin membrane more efficiently than CHAPS or Triton X‐100 …”
Section: Discussionmentioning
confidence: 99%
“…For example, the node of Ranvier may offer undiscovered autoantigens . However, those therapeutically and pathophysiologically relevant proteins are often lost in early steps . Therefore, we adapted the steps of the immunoblotting approach and rescued refractory proteins in this study.…”
Section: Introductionmentioning
confidence: 99%
“…In a context of cell signal transduction, membrane proteins additionally can be key components (including transmembrane receptors), and this brings further attention to detergent considerations [14]. In particular, this includes a requirement to retain the solubility of hydrophobic proteins, while also maintaining protein-protein partnerships [15,16]. One non-ionic detergent frequently suggested as a potentially advantageous choice for this challenge is octyl beta-D-glucoside (OBG).…”
Section: Editorialmentioning
confidence: 99%
“…33,34 A range of experimental methods are applied to solubilize and separate individual proteins based on their biochemical characteristics before identification by mass spectrometry. 35,36 For P. falciparum, these have included two-dimensional gel electrophoresis, 37 membrane solubilization and purification, 38 and surface biotinylation 39,40 (Fig. 3).…”
Section: Proteomicsmentioning
confidence: 99%