Določitev vzročnih genetskih različic pri prirojeni eritrocitozi s sekvenciranjem naslednje generacije in funkcionalna opredelitev izbranih različic

Kristan, Aleša

Določitev vzročnih genetskih različic pri prirojeni eritrocitozi s sekvenciranjem naslednje generacije in funkcionalna opredelitev izbranih različic
ID Kristan, Aleša (Avtor), ID Debeljak, Nataša (Mentor) Več o mentorju... Povezava se odpre v novem oknu

, ID Preložnik Zupan, Irena (Komentor)

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Izvleček

Uvod: Eritrocitoza je bolezensko stanje, pri katerem pride do povečanega števila eritrocitov, kar sovpada s povišanimi vrednostmi hemoglobina in/ali hematokrita v krvni sliki. Najpogostejši vzroki za eritrocitozo so pridobljeni, medtem ko je prirojena eritrocitoza redka oblika z znanimi vzroki v devetih različnih genih (EPOR, VHL, EGLN1, EPAS1, EPO, HBB, HBA1, HBA2 in BPGM), ki povzročajo osem različnih tipov prirojene eritrocitoze (ECYT 1-8). Zaradi raznolike etiologije je diagnostika eritrocitoze zahtevna, vzrok pa v večini primerov ostaja idiopatski. Molekularno-genetska diagnostika prirojene eritrocitoze v Sloveniji do sedaj še ni bila uveljavljena, zato je veliko bolnikov s sumom na prirojeno eritrocitozo ostalo brez potrjenega genetskega vzroka in v nekaterih primerih so bili tudi neustrezno zdravljeni. Cilji: Namen raziskave je bil poiskati genetski vzrok, povezan z razvojem eritrocitoze, pri slovenskih bolnikih, pri katerih obstaja sum na prirojeno eritrocitozo. Prav tako smo ocenili vpliv odkrite nove genetske različice na razvoj eritrocitoze. Metode: S sistematičnim pregledom literature in uporabo različnih in silico orodij za analizo molekularnih poti vključenih v eritropoezo, smo izbrali kandidatne gene in regije za tarčno sekvenciranje. Z novo vzpostavljenim nacionalnim diagnostičnim algoritmom je bilo opredeljenih 28 bolnikov s simptomi prirojene eritrocitoze, ki so bili vključeni v raziskavo, vključno s tremi družinami z dvema zdravima družinskimi članoma. Vzorci so bili analizirani s tarčnim sekvenciranjem naslednje generacije (NGS). Izbrana nova genetska različica je bila nadalje funkcionalno opredeljena z lokalizacijo različice na 3D strukturi proteina, analizo izražanja proteina s kvantitativnim prenosom western in analizo aktivnosti proteina z uporabo luciferaznega poročevalskega testa. Rezultati: Za tarčni NGS je bilo izbranih 39 genov, ki so povezani z eritrocitozo in presežkom železa v telesu. S tarčnim NGS 28-ih bolnikov smo odkrili eno znano patogeno različico v genu EPAS1, c.1609G>A (p.(Gly537Arg)), in štiri različice neznanega pomena (ang. variant of unknown significance, VUS) v genih EGLN1, JAK2, EPAS1 in SH2B3. V eni družini smo ugotovili tudi dve različici z nizko frekvenco v populaciji (< 5 %), v genih EGLN1 in JAK2. Poleg tega smo opazili visoko pojavnost prenašalcev patogenih različic v genu HFE. Različica c.1072C>T (p.(Pro358Ser)) v genu EGLN1 je ko-segregirala z boleznijo pri več družinskih članih, imela je visoko napoved patogenosti ter ni bila opisana v literaturi in klinični zbirki podatkov, zato je bila izbrana za dodatne funkcionalne analize. Lokalizacija na 3D strukturi proteina je pokazala, da se različica nahaja v aktivnem centru proteina in lahko vpliva na njegovo aktivnost. Rezultati kvantitativnega prenosa western so pokazali statistično pomembno (P < 0,0001) zmanjšano izražanje proteina EGLN1 z različico c.1072C>T (p.(Pro358Ser)), v primerjavi z nativnim proteinom. Oba rezultata nakazujeta na zmanjšano aktivnost EGLN1. Z luciferaznim poročevalskim testom nismo potrdili vpliva različice c.1072C>T (p.(Pro358Ser)) na zmanjšano aktivnost EGLN1. Zaključki: S tarčnim NGS smo uspešno potrdili genetski vzrok za eritrocitozo pri enem bolniku, prvem slovenskem bolniku s prirojeno eritrocitozo (ECYT4). Poleg tega smo identificirali štiri VUS v genih EGLN1, JAK2, EPAS1 in SH2B3, pri tem smo VUS v genu EGLN1 izbrali za nadaljnjo funkcionalno opredelitev. Rezultati funkcionalnih analiz so pokazali lokacijo različice v aktivnem mestu proteina EGLN1 in vpliv na izražanje proteina, ne pa tudi na aktivnost. Za opredelitev vpliva različice na delovanje proteina in nadaljnjo uravnavanje izražanja s hipoksijo induciblnih tarčnih genov so potrebne dodatne analize.

Jezik:	Slovenski jezik
Ključne besede:	eritrocitoza, sekvenciranje naslednje generacije (NGS), genetske različice, funkcionalna analiza, eritropoeza, metabolizem železa
Vrsta gradiva:	Doktorsko delo/naloga
Organizacija:	MF - Medicinska fakulteta
Leto izida:	2023
PID:	20.500.12556/RUL-151710
Datum objave v RUL:	18.10.2023
Število ogledov:	877
Število prenosov:	9
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Izvleček:
Jezik:	Angleški jezik
Naslov:	Next generation sequencing approach for detecting causal genetic variants for hereditary erythrocytosis and functional assessment of selected variants
Background: A condition of an increased number of erythrocytes is termed erythrocytosis and coincides with elevated haemoglobin and/or haematocrit levels in the blood picture. The most common causes for erythrocytosis are acquired, while hereditary erythrocytosis is a rare condition with known causes in nine different genes (EPOR, VHL, EGLN1, EPAS1, EPO, HBB, HBA1, HBA2, and BPGM) that lead to eight different types of hereditary erythrocytosis (ECYT 1-8). Due to diverse aetiology, the diagnostics is problematic and the cause remains idiopathic in the majority of the cases. The molecular-genetic diagnostics of hereditary erythrocytosis was not yet established in Slovenia, hence many patients suspected of hereditary erythrocytosis remained without genetic cause and in some cases were also inappropriately treated. Aims: The aim of this study was to find a genetic cause associated with the development of erythrocytosis in Slovenian patients suspected of hereditary erythrocytosis. We also evaluated the effect of the identified novel genetic variant on the development of erythrocytosis. Methods: Selection of genes and regions for targeted genetic testing was performed with systematic revision of the literature and with analysis of molecular pathways, involved in erythropoiesis, using different in silico tools. A newly established national diagnostic algorithm identified 28 patients with symptoms of hereditary erythrocytosis, that were included in the study, including three families with two healthy family members. Samples were analyzed using a targeted next-generation sequencing (NGS). The selected novel genetic variant was further functionally assessed with localization of the variant on a 3D protein structure, protein expression analysis with quantitative western blotting, and protein activity analysis using a luciferase reporter assay. Results: 39 genes with association with erythrocytosis and iron overload were selected for NGS analysis. Targeted NGS of 28 patients identified one known pathogenic variant in the EPAS1 gene, c.1609G>A (p.(Gly537Arg)), and four variants of unknown significance (VUS) in the EGLN1, JAK2, EPAS1, and SH2B3 genes. In one family we also identified two low-frequency variants (< 5%) in the EGLN1 and JAK2 genes. Additionally, we observed a high incidence of variant carriers for pathogenic variants in the HFE gene. VUS c.1072C>T (p.(Pro358Ser)) in the EGLN1 gene was observed in strong co-segregation with a disease in multiple family members, had high pathogenicity prediction scores, and was not reported in the literature and clinical database, therefore this variant was further functionally assessed. Localization on a 3D protein model showed that the variant is positioned in an active site of the protein and may affect protein activity. Protein quantification results showed statistically significant (P < 0.0001) reduced protein expression of EGLN1 with variant c.1072C>T (p.(Pro358Ser)) in comparison to the wild-type protein. Both results implicate reduced activity of the protein. However, the luciferase reporter assay did not confirm the effect of variant c.1072C>T (p.(Pro358Ser)) on the EGLN1 activity. Conclusions: With targeted NGS we successfully confirmed the genetic cause for erythrocytosis in one patient, the first Slovenian patient with hereditary erythrocytosis (ECYT4). Additionally, we identified four VUS in the EGLN1, JAK2, EPAS1, and SH2B3 genes, among them VUS in the EGLN1 gene was selected for further functional assessment. Results of functional tests showed the position of the variant in an active site of EGLN1 protein and an effect on EGLN1 expression, but not on EGLN1 activity. However, further tests are necessary to review the effect of the variant on protein function and further transcription regulation of hypoxia-inducible targets.
Ključne besede:	erythrocytosis, next-generation sequencing (NGS), genetic variants, functional analysis, erythropoiesis, iron metabolism

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