Detergents: Friends not foes for high‐performance membrane proteomics toward precision medicine

Zhang, Xi

doi:10.1002/pmic.201600209

Cited by 10 publications

(14 citation statements)

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%

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Completing the Immunological Fingerprint by Refractory Proteins: Autoantibody Screening via an Improved Immunoblotting Technique

Moritz

Tholance

Rosier

et al. 2019

Proteomics Clinical Apps

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Purpose: Identifying autoantigens of serological autoantibodies requires expensive methods, such as protein microarrays or IP+MS. Thus, sera are commonly pre-screened for interesting immunopatterns via immunocytochemistry/immunohistochemistry. However, distinguishing immunopatterns can be difficult and intracellular antigens are less accessible. Therefore, a simple and cheap immunoblot screening able to distinguish immunopatterns and to detect refractory proteins is presented. Experimental Design: Five steps of immunoblotting-based autoantigen screening are revised: (1) choice of protein source, (2) protein extraction, (3) protein separation, (4) protein transfer, (5) antigen detection. Thereafter, 52 patients' sera with chronic inflammatory demyelinating polyneuropathy (CIDP) and 45 controls were screened. Results: The protein source impacts the detected antigen set. Steps 2-4 can be adapted for refractory proteins. Furthermore, longitudinal cutting of protein lanes saves ࣙ75% of time and material and allows for exact comparison of band patterns. As the latter are individually specific and temporarily constant, we call them "immunological fingerprints". In a proof-of-principle, a 155 kDa immunoband was detected with two anti-neurofascin-155-positive CIDP sera and two further immunobands (120/220 kDa) specific to a subgroup of 3-6 of 52 CIDP patients. Conclusions and Clinical Relevance: Adapted immunoblotting is a cheap and simple method for accurate serum screening including refractory and intracellular antigens.

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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%

Completing the Immunological Fingerprint by Refractory Proteins: Autoantibody Screening via an Improved Immunoblotting Technique

Moritz

Tholance

Rosier

et al. 2019

Proteomics Clinical Apps

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“…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%

Optimizing Workflows for LC/MS Analysis of Co-Immunoprecipitated Protein Complexes – “Soap Opera (tions)”

Held¹,

Wojchowski²

2018

J Proteomics Bioinform

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“…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%

Vaccine candidate discovery for the next generation of malaria vaccines

et al. 2017

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SummaryAlthough epidemiological observations, IgG passive transfer studies and experimental infections in humans all support the feasibility of developing highly effective malaria vaccines, the precise antigens that induce protective immunity remain uncertain. Here, we review the methodologies applied to vaccine candidate discovery for Plasmodium falciparum malaria from the pre‐ to post‐genomic era. Probing of genomic and cDNA libraries with antibodies of defined specificities or functional activity predominated the former, whereas reverse vaccinology encompassing high throughput in silico analyses of genomic, transcriptomic or proteomic parasite data sets is the mainstay of the latter. Antibody‐guided vaccine design spanned both eras but currently benefits from technological advances facilitating high‐throughput screening and downstream applications. We make the case that although we have exponentially increased our ability to identify numerous potential vaccine candidates in a relatively short space of time, a significant bottleneck remains in their validation and prioritization for evaluation in clinical trials. Longitudinal cohort studies provide supportive evidence but results are often conflicting between studies. Demonstration of antigen‐specific antibody function is valuable but the relative importance of one mechanism over another with regards to protection remains undetermined. Animal models offer useful insights but may not accurately reflect human disease. Challenge studies in humans are preferable but prohibitively expensive. In the absence of reliable correlates of protection, suitable animal models or a better understanding of the mechanisms underlying protective immunity in humans, vaccine candidate discovery per se may not be sufficient to provide the paradigm shift necessary to develop the next generation of highly effective subunit malaria vaccines.

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Detergents: Friends not foes for high‐performance membrane proteomics toward precision medicine

Cited by 10 publications

References 178 publications

Completing the Immunological Fingerprint by Refractory Proteins: Autoantibody Screening via an Improved Immunoblotting Technique

Completing the Immunological Fingerprint by Refractory Proteins: Autoantibody Screening via an Improved Immunoblotting Technique

Optimizing Workflows for LC/MS Analysis of Co-Immunoprecipitated Protein Complexes – “Soap Opera (tions)”

Vaccine candidate discovery for the next generation of malaria vaccines

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