Smart blood spots for whole blood protein analysis

Skjærvø, Øystein; Halvorsen, Trine Grønhaug; Reubsaet, Léon

doi:10.1039/c8an00317c

Cited by 16 publications

(32 citation statements)

References 29 publications

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“…Functionalization using HEMA-VDM: For the HEMA-VDM functionalization, the procedure published by Skjaervø et al [29,[36][37][38] was slightly modified and used. In short, the fibers on the paper discs were first silanized by applying 10 µL of freshly prepared silanizing solution (this is a mixture of 2.5 mg DPPH, 330 mg DMF and 172 mg γ-MAPS prepared in a glass vial).…”

Section: Functionalization Of Paper Discs and Protein Immobilizationmentioning

confidence: 99%

“…Prior to injection, clean-up was carried out on 100 µL of the sample using in-housemade solid phase extraction as described by [29]. After drying, the residue was reconstituted using 100 µL 0.1% formic acid and transferred to the injection vial.…”

Section: Serum Digestion On Functionalized Paper With Immobilized Trypsinmentioning

confidence: 99%

“…Here, cellulose was first silanized, then functionalized through the polymerization of 2hydroxyethyl methacrylate (HEMA) and 2-vinyl-4,4-dimethylazlactone (VDM), allowing trypsin to bind covalently to paper [29]. Besides this protocol, there are other possibilities to bind proteins covalently to paper [30][31][32][33][34], among which is also the simple KIO 4 -mediated oxidation of cellulose to create two aldehyde groups per cellulose unit, allowing subsequent protein binding.…”

Section: Introductionmentioning

confidence: 99%

“…The long-term goal of our research is to simplify MS-based protein analysis from dried matrix samples (such as DBS), and we aim to integrate time-consuming procedures within the sampling device for a prompt start to the sample preparation upon sample collection [29,[35][36][37][38].…”

Section: Introductionmentioning

confidence: 99%

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Next-Generation Dried Blood Spot Samplers for Protein Analysis: Describing Trypsin-Modified Smart Sampling Paper

et al. 2021

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This paper describes smart sampling paper to be used for bottom-up protein analysis. Four different manners to immobilize trypsin on cellulose were evaluated. Untreated paper, potassium-periodate-functionalized paper (with and without post-immobilization reduction) and 2-hydroxyethyl methacrylate (HEMA)/2-vinyl-4,4-dimethylazlactone (VDM)-functionalized paper were all used to immobilize trypsin. For the evaluation, Coomassie Brilliant Blue staining of proteins on paper and the BAEE trypsin activity assay needed to be modified. These methods allowed, together with data from mass spectrometric analysis of cytochrome C digestions, us to acquire fundamental insight into protein binding, and trypsin action and activity on paper. All functionalized discs bind more protein than the untreated discs. Protein binding to functionalized discs is based on both adsorption and covalent binding. Trypsin immobilized on potassium-periodate-functionalized discs exhibits the highest trypsin activity when using cytochrome C as substrate. It is proven that it is trypsin attached to paper (and not desorbed trypsin) which is responsible for the enzyme activity. The use of discs on complex biological samples shows that all functionalized discs are able to digest diluted serum; for the best-performing disc, HEMA-VDM functionalized, up to 200 high-confidence proteins are qualified, showing its potential.

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Section: Functionalization Of Paper Discs and Protein Immobilizationmentioning

confidence: 99%

Section: Serum Digestion On Functionalized Paper With Immobilized Trypsinmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

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Next-Generation Dried Blood Spot Samplers for Protein Analysis: Describing Trypsin-Modified Smart Sampling Paper

et al. 2021

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“…Our group has been working with the concept of smart sampling in combination with MS determination since 2017 [45]. This concept is based on the covalent binding of trypsin to cellulose allowing a DBS sampler to start with the digestion step at the moment of sampling [46][47][48][49]. This smart sampler does not compromise the ease of sampling as the format remains practically unchanged.…”

Section: Introductionmentioning

confidence: 99%

Smart proteolysis samplers for pre‐lab bottom‐up protein analysis – Performance of on‐paper digestion compared to conventional digestion

Nguyen

Halvorsen

Thiede

et al. 2022

Separation Science Plus

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Here the relation between digestion of proteins by trypsin covalently bound to paper and trypsin in‐solution is investigated. The trypsin acting on paper is covalently bound. A trypsin concentration of 0.5% (w/v) results in the highest digestion activity of all concentrations tested. Additionally, it can be seen that trypsin on‐paper has retained approx. 50% of its activity. Unlike trypsin in‐solution, the stability of the smart proteolysis samplers was regarded to be stable for at least four months when kept refrigerated. Autolysis was very small for covalently bound trypsin: less than 2% compared to in‐solution trypsin. Proteomic analysis of diluted human serum showed more protein identifications (214) in‐solution digestions than on‐paper digestions (76). Also, higher coverage for the in‐solution digestion was obtained. Those proteins identified after on‐paper digestion with no or few disulfide bonds seem to have more similar sequence coverages compared to those identified after in‐solution digestion. Smart samplers allow the determination of at least 70–75 proteins without performing the overnight digestion. All in all, trypsin covalently bound to paper shows to retain high proteolytic activity and is a stable alternative for conventional digestions. In this way, smart proteolytic samplers show their feasibility in pre‐lab sample preparation.

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Is this the end of dried blood spots as we know it?

Halvorsen

Reubsaet

2023

Analytical Science Advances

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In 2017 integrated sampling and sample preparation for simplified liquid chromatography‐mass spectrometry analysis of proteins from dried blood spots were introduced. The concept, called smart samplers or smart sampling, enables proteolysis or affinity clean‐up, two common sample preparation steps in liquid chromatography‐mass spectrometric bioanalysis of proteins, to start at the moment of sampling. The idea is to utilize the time for sampling and drying to perform these time‐consuming and labour‐intensive steps. Hence, only a simplified sample preparation is necessary after the arrival of the sample in the lab. In this perspective, we present an overview of the smart sampling approach where the conventional protein analysis workflow is reshuffled to start already prior to arrival in the lab. In addition, we present a thorough discussion of integrating sample preparation steps such as proteolysis or affinity capture in the sampling. Finally, in the end, we try to answer the question if conventional dried blood spots will become obsolete in the future.

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Smart blood spots for whole blood protein analysis

Cited by 16 publications

References 29 publications

Next-Generation Dried Blood Spot Samplers for Protein Analysis: Describing Trypsin-Modified Smart Sampling Paper

Next-Generation Dried Blood Spot Samplers for Protein Analysis: Describing Trypsin-Modified Smart Sampling Paper

Smart proteolysis samplers for pre‐lab bottom‐up protein analysis – Performance of on‐paper digestion compared to conventional digestion

Is this the end of dried blood spots as we know it?

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