2017
DOI: 10.1016/j.jprot.2016.07.028
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Secretome profiling of apheresis platelet supernatants during routine storage via antibody-based microarray

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Cited by 13 publications
(14 citation statements)
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“…showing that these proteins had more than two-fold increase in their expression profiles in the "thrombinactivated" vs "resting" platelets. We recovered a high overlap of proteins members with the kinome family reported already by other proteomic analyses, [20][21][22][23][24][25][26][27][28][29][30] that are also indexed in many other research studies related to the proteomic profiling of agonists activated platelets, such as the "Adhesome" and "Platelet Web" databases, as described later in the results section. Other major pathways predicted by IPA to be up-regulated in the proteome of "thrombin-activated platelets" were mapped to the cytoskeleton, actin and RhoA mediated cellular signaling ( Figure 18).…”
Section: Figure 14mentioning
confidence: 86%
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“…showing that these proteins had more than two-fold increase in their expression profiles in the "thrombinactivated" vs "resting" platelets. We recovered a high overlap of proteins members with the kinome family reported already by other proteomic analyses, [20][21][22][23][24][25][26][27][28][29][30] that are also indexed in many other research studies related to the proteomic profiling of agonists activated platelets, such as the "Adhesome" and "Platelet Web" databases, as described later in the results section. Other major pathways predicted by IPA to be up-regulated in the proteome of "thrombin-activated platelets" were mapped to the cytoskeleton, actin and RhoA mediated cellular signaling ( Figure 18).…”
Section: Figure 14mentioning
confidence: 86%
“…The "in solution" digestion with three enzymes (trypsin/LysC/Glu-C), enabled the extraction of peptides from the total platelet proteome, including the membrane-derived and microvesicles contained in the releasates, as reported previously by other studies on platelets proteomics. [20][21][22][23][24][25][26][27][28][29][30] The extracted peptides were subjected to nano LC/MS/MS sequencing on a Q Exactive quadrupole orbitrap mass spectrometer, as summarized in the protocol shown in Figure 1. The label-free proteomics analysis employed the label free quantification (LFQ) module provided by PEAKS 8.5 (Bioinformatics Solutions Inc.), In addition, the changes in the protein expression profiles were complemented by an additional analysis involving the Scaffold and per SPECtives software (Proteome Software Inc.).…”
Section: Development Of a Workflow For Implementing The Label-free Phmentioning
confidence: 99%
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“…Platelets are non-nucleated cells derived from very large pre-cursor cells called megakaryocytes that reside in the bone marrow. During their development, platelets obtain large numbers of storage granules that contain different growth factors, cytokines, and hormones required for activating acute inflammation, which is the first stage of wound repair [11,12,14,37,38] . Platelet activation is a highly regulated process that culminates in degranulation, or the release of granule contents [12,[39][40][41][42][43] .…”
Section: Salient Roles Of Blood Components In Wound Repairmentioning
confidence: 99%