Pregled bibliografske jedinice broj: 1094574
Exosomes, a Challenging Target for Quantitative Proteomics
Exosomes, a Challenging Target for Quantitative Proteomics // Book of Abstracts of 30th MassSpec-Forum Vienna
Beč, Austrija, 2019. str. 31-31 (poster, međunarodna recenzija, sažetak, znanstveni)
CROSBI ID: 1094574 Za ispravke kontaktirajte CROSBI podršku putem web obrasca
Naslov
Exosomes, a Challenging Target for Quantitative
Proteomics
Autori
Hixson, Douglas ; Begić, Marija ; Šrajer Gajdošik, Martina ; Callanan, Helen ; Aliotta, Jason ; Brilliant, Kate ; Quesenberry, Peter ; Josić, Djuro
Vrsta, podvrsta i kategorija rada
Sažeci sa skupova, sažetak, znanstveni
Izvornik
Book of Abstracts of 30th MassSpec-Forum Vienna
/ - , 2019, 31-31
Skup
MassSpec-Forum 2019
Mjesto i datum
Beč, Austrija, 19.02.2019. - 20.02.2019
Vrsta sudjelovanja
Poster
Vrsta recenzije
Međunarodna recenzija
Ključne riječi
Exosomes ; Quantitative proteomics ; Liver perfusion
Sažetak
Microvesicles released by many cell types are a heterogeneous population of large (100- 1000nm) and small vesicles called exosomes (30-100nM). Interest in microvesicles has blossomed since reports of their ability to reprogram cellular phenotypes via the horizontal transfer of mRNA, proteins or microRNAs. To determine if MV from other tissues could induce tissue specific genes, the experiments with liver tissue from mice as MV donor and rat BMC as target cells were performed. When analyzed by RT-PCR, transcripts for both rat and mouse albumin were detected suggesting MV mediated transfer of functional albumin mRNA as well as transcriptional activators for the rat albumin gene [2};. Additionally, we are searching for alternative methods to generate MV from intact liver. To obtain a closer approximation to normal liver, MV were collected from medium conditioned by recirculation through an isolated perfused liver. TEM examination revealed an unexpectedly clean preparation of MV ranging from 40nm to 800nm in diameter. When MVs were collected by perfusion of an isolated liver after injury, from a rat treated with 500mg/Kg acetaminophen, striking differences were observed in the size distribution of MV. To determine if there were also differences in composition, 15 ug of MV collected from normal and acetaminophen treated rat livers were solubilized, digested with trypsin and analyzed by LC-ESI-MS/MS. In addition to standard methods for sample preparations and tryptic digestion, a so-called “in gel digestion method” for tryptic hydrolyisis of microvesicle samples was applied [2]. By use of this approach, additional very hydrophobic proteins were identified, especially in MV samples that were shed by injures liver. These results revealed marked differences in MV proteomes. Of the 200 proteins identified between the two samples, 67 and 100 were unique to normal and acetaminophen treated livers, respectively and 53 were held in common. While MV from normal liver had a preponderance of phase 1 (CYP450s) and phase II detoxification enzymes, those from acetaminophen treated livers were enriched for annexins, signaling proteins, and membrane receptors, transporters and enzymes. These results suggest the possibility of defining different types of liver injury by the proteomic signature of MV collected by perfusion or shed into the serum.
Izvorni jezik
Engleski
Znanstvena područja
Kemija, Biotehnologija u biomedicini (prirodno područje, biomedicina i zdravstvo, biotehničko područje)
POVEZANOST RADA
Ustanove:
Sveučilište u Osijeku - Odjel za kemiju,
Sveučilište u Rijeci - Odjel za biotehnologiju
