L’analisi di espressione dei retrovirus Human T-cell lymphotropic viruses (HTLV-1 e 2) durante il processo di infezione è essenziale per capire l’influenza che i prodotti dei geni virali hanno sui processi di proliferazione, ciclo e signalling cellulari. Studi recenti condotti su cellule infettate con HTLV-1 hanno ermesso di delineare la cinetica di espressione dei diversi trascritti virali. Per quanto concerne HTLV-2, il profilo di espressione degli mRNA virali in cellule infettate risulta ancora poco studiato e le relative cinetiche non sono state ancora delineate. Scopo di questo studio è stato quindi quello di analizzare l’espressione dei diversi trascritti di HTLV-2 mediante la messa a punto di analisi real time RT-PCR per la loro determinazione quantitativa. In particolare sono state studiate e quantificate le cinetiche di espressione dei trascritti di HTLV-2 in linee cellulari infettate e in linfociti da sangue periferico (PBMC) provenienti da pazienti infetti. In modo analogo ad altri retrovirus, HTLV-2 esprime diversi prodotti genici dalla stessa regione codificante, attraverso diverse strategie che sottointendono un complesso pattern di splicing alternativo. L’espressione di HTLV-2 è basata su tre principali classi di mRNA: a) “unspliced” mRNA, che codifica per le proteine Gag, Pol e Proteasi; b) “singly” spliced mRNA che codifica per Env e per le proteine accessorie p28 e p22/p20; c) “doubly spliced” mRNA che codifica per le proteine Tax, Rex e le proteine accessorie p10, p11 ed 1-2-B. Recentemente inoltre è stato descritto un nuovo prodotto proteico, APH-2, che viene codificato dallo strand negativo di HTLV-2 e sembra essere coinvolto nei processi di silenziamento trascrizionale del virus in cellule infettate. Il profilo di espressione e le cinetiche dei diversi trascritti virali sono stati quantificati mediante la metodica di Real Time RT-PCR, utilizzando sonde e primers specifici per le giunzioni di splicing. Il profilo temporale di ogni trascritto di HTLV-2 è stato studiato utilizzando tre diversi sistemi cellulari: linee stabilmente infettate, cellule trasfettate in modo transiente, e infine PBMC provenienti da soggetti infettati da HTLV- 2B messi in colturea e stimolati con IL-2. I risultati ottenuti in questo studio hanno portato alla quantificazione di tutti i trascritti virali di HTLV-2. Sono stati inizialmente riscontrati diversi livelli di espressione di env nei due sottotipi HTLV-2 A e B. La diversa espressione del trascritto env in linee cellulari stabilente infettate, ha indotto ad approfondire il complesso meccanismo di splicing tra gli esoni 1 e 2, portando all’identificazione di un nuovo sito accettore di splicing (3’SS). Si è potuto così determinare che questo nuovo sito accettore viene utilizzato nell’espressione del trascritto env “singly splicing” e dei trascritti bicistronici tax/rex, p10/p11 e 1-2-B “doubly splicing” derivati da splicing alternativo all’interno della regione genica pX di HTLV-2. I risultati sperimentali hanno quindi permesso di evidenziare che il nuovo sito 3’SS è presente in entrambi i sottotipi A e B di HTLV-2 e che la nuova isoforma di env, chiamata env 1-2b, è preferenzialmente espressa nel sottotipo 2B mentre nel sottotipo 2A l’espressione di env utilizza più efficientemente il sito canonico di splicing. L’analisi della cinetica di espressione del mRNA totale, ha mostrato un andamento caratterizzato da una bassa trascrizione iniziale, seguita da un aumento con un progressivo picco di espressione dopo 21-24 ore dall’inizio della coltura. Il trascritto “full lenght” gag/pol risulta essere il più espresso durante il periodo analizzato, comportandosi come un gene tardivo e raggiungendo quindi un picco di espressione dopo 21-48 ore. L’env canonico è espresso a livelli molto bassi nelle linee stabilmente infettate e non e’ rilevabile in PBMC di pazienti infettati da HTLV-2B. Al contrario, l’isoforma env 1-2b viene efficientemente espressa, sia in linee cellulari che in PBMC ex-vivo e presenta un profilo di espressione tardivo seguito da un graduale e costante aumento, raggiungendo il picco massimo di espressione tra 21 e 48 ore. Infine il trascritto di regolazione tax/rex viene espresso precocemente da HTLV-2B sia in linee stabilmente infettate che in ex-vivo PBMC. Le cinetiche del trascritto 1-2-B indicano che questo gene viene espresso ad alti livelli negli intervalli di tempo precoci mentre il mRNA per le proteine accessorie p10 e p11 risulta essere poco espresso o inferiore alla soglia di detezione. Tra gli mRNA che subiscono “singly splicing” e che codificano per le proteine accessorie, l’isoforma p28,p22/p20-II è maggiormente espressa nei due sottotipi HTLV-2A e B rispetto all’isoforma p28, p22/p20-I. Il trascritto APH-2 viene espresso ad alti livelli sia in cellule stabilmente infettate che in cellule trasfettate e presenta un andamento tardivo in questi sistemi cellulari. Tuttavia nei PBMC ottenuti da pazienti infetti non e' stato possibile determinarne un chiaro pattern di espressione in quanto questo trascritto risulta essere molto variabile. Questo studio ha messo in evidenza che i trascritti di HTLV-2 presentano cinetiche di espressione specifiche e diversificate. I risultati ottenuti hanno permesso di descrivere un preciso pattern di produzione temporale degli mRNA, con geni precoci quali tax/rex e 1-2-B e geni tardivi quali gag/pol, env e 28,p22/p20-II. L’espressione precoce di tax/rex indica che questa proteina è necessaria nelle fasi iniziali del ciclo virale al fine di transattivare e regolare i geni virali e cellulari. I geni strutturali gag/pol e env sono invece espressi tardivamente quando i livelli d’espressione dei geni precoci sono in fase di dimunuizione, il che indica quindi un chiaro “switch” temporale tra geni precoci e tardivi. Questo studio ha inoltre evidenziato un nuovo sito accettore di splicing alternativo nella regione pX di HTLV-2. In conclusione, questo studio ha permesso di stabilire che i livelli dei geni di HTLV-2 e le loro cinetiche di espressione sono strettamente regolati. Inoltre, queste ricerche hanno messo in evidenza che l’utilizzo di nuovi siti accettori gioca un ruolo fondamentale nell’ espressione preferenziale di proteine virali specifiche alle diverse fasi del ciclo virale di HTLV-2.
The analysis of HTLV expression during the infection process is essential to understand the influence of viral gene products on proliferation, cell cycle and signalling. Recent studies carried out on HTLV-1-infected cells have provided information on the relative abundance and timing of expression of different viral transcripts. In the case of HTLV-2, very little information has been so far obtained on the profile of viral gene expression in infected cells, and the kinetics of transcript expression have not yet been investigated. The aim of the study was to further investigate HTLV-2 transcripts expression, by developing new quantitative analyses to measure the levels of expression of different HTLV-2 mRNAs. In particular the kinetics of HTLV-2 transcripts at different stages of virus gene expression and their quantitation in infected cell lines and in PBMCs from infected subjects, have been evaluated. Similarly to other retroviruses, HTLV-2 expresses multiple gene products from the same coding region by choosing different strategies, including a complex pattern of alternative splicing. HTLV-2 expression produces three major classes of mRNAs: unspliced mRNA for Gag, Protease and Pol proteins; singly spliced mRNAs for Env and accessory proteins p28 and p22/p20; and doubly spliced mRNAs for the regulatory Tax, Rex and the accessory p10, p11 and 1-2-B proteins. More recently, the new APH-2 protein coded by the negative strand of HTLV-2, and possibly involved in the transcriptional silencing of the virus in infected cells was described. The expression profile and kinetics of the different transcripts were analysed by RT-PCR assays using a series of splice-junction-specific primers and probes. The time courses of each HTLV-2 transcript in three different cellular systems, namely stably infected cells lines, transiently transfected cells and ex-vivo IL-2 stimulated PBMCs from infected subjects were investigated. The results obtained led to the quantitation of all known HTLV-2 mRNAs. Preliminary data showed different levels of env transcript in HTLV-2 subtypes A and B. Evidence for a differential env expression in HTLV-2B stably infected cells, prompted further investigation on the complex pattern of splicing between exons 1 and 2 and allowed the identification of a novel 3’ acceptor site (SS) of splicing. This novel 3’SS is used to express alternative spliced isoforms within the pX terminal region of HTLV-2, including the singly spliced env and the three doubly spliced bicistronic tax/rex, p10/p11 and 1-2-B transcripts. Results demonstrated that the novel 3’SS was utilised in both HTLV-2 subtypes, and that the novel env isoform, named env 1-2b, was preferentially expressed in 2B subtypes, while 2A subtypes used more efficiently the canonical splice site. The kinetics of total mRNA HTLV-2 expression in these three cellular systems presented a general pattern characterised by an initial low transcript level and a subsequent increase to reach a peak of expression after 21-24 hours in culture. The full length gag/pol mRNA was the most abundant one during the time course, and behaved as a late gene that peaked after 21 to 48 hours. The canonical env transcript was expressed at very low rates in stably infected cells, and it was undetectable in PBMCs from infected subjects and in cells transfected with the HTLV-2 proviral clone. By contrast, env 1-2b isoform was efficiently expressed in stably infected cells as well as in ex-vivo infected PBMCs, behaving as a late gene showing a gradual and steady increase in copy number and reaching maximum expression at 21 to 48 hours. The regulatory tax/rex gene was expressed early and with a high/intermediate transcription rate in HTLV-2B subtypes in both stably infected cells and ex-vivo PBMCs. In this study the kinetics of expression of the yet unkwnon 1-2-B gene was investigated and found to be expressed at high levels at early time points, whereas the doubly spliced mRNA of accessory p10/p11 genes were poorly expressed or under detection limit. Among the singly spliced mRNAs coding for other accessory proteins, the p28, p22/p20-II isoform was found to be highly expressed in both HTLV-2 A and B subtypes as compared to its alternative p28, p22/p20-I form. The APH-2 negative transcript was efficiently expressed at high levels in both stably infected and transfected cells and behaved as a late gene. However, in ex-vivo PBMCs its expression level and kinetics pattern appeared to be variable and a clear pattern of expression was not assessed. In conclusion, this study demonstrated that HTLV-2 transcripts of both A and B subtypes are differentially expressed. A temporal pattern of mRNA production, with early, tax/rex and 1-2-B and late, gag/pol, env, p28,p22/p20-II genes was established. The tax/rex early expression indicates that this protein is necessary at the beginning of the viral cycle to transactivate and regulate viral and cellular genes. Most structural genes were expressed late when the transcription of early genes was already decreasing, thus showing that a temporal switch was occurring between early to late genes production. This study also provided new clues on the selective use of alternative 3’SS within the pX region of HTLV-2 for both subtypes A and B. Overall these findings indicate that the control of HTLV-2 viral gene expression is highly regulated both in its kinetics and expression. Moreover, it suggests that the use of multiple acceptor sites might play an important role on the preferential expression of specific proteins in the different phases of the viral cycle.
Study of Human T-Lymphotropic Virus type 2 mRNA kinetics of expression and identification of a novel splicing site
BENDER, Cecilia
2010-01-01
Abstract
The analysis of HTLV expression during the infection process is essential to understand the influence of viral gene products on proliferation, cell cycle and signalling. Recent studies carried out on HTLV-1-infected cells have provided information on the relative abundance and timing of expression of different viral transcripts. In the case of HTLV-2, very little information has been so far obtained on the profile of viral gene expression in infected cells, and the kinetics of transcript expression have not yet been investigated. The aim of the study was to further investigate HTLV-2 transcripts expression, by developing new quantitative analyses to measure the levels of expression of different HTLV-2 mRNAs. In particular the kinetics of HTLV-2 transcripts at different stages of virus gene expression and their quantitation in infected cell lines and in PBMCs from infected subjects, have been evaluated. Similarly to other retroviruses, HTLV-2 expresses multiple gene products from the same coding region by choosing different strategies, including a complex pattern of alternative splicing. HTLV-2 expression produces three major classes of mRNAs: unspliced mRNA for Gag, Protease and Pol proteins; singly spliced mRNAs for Env and accessory proteins p28 and p22/p20; and doubly spliced mRNAs for the regulatory Tax, Rex and the accessory p10, p11 and 1-2-B proteins. More recently, the new APH-2 protein coded by the negative strand of HTLV-2, and possibly involved in the transcriptional silencing of the virus in infected cells was described. The expression profile and kinetics of the different transcripts were analysed by RT-PCR assays using a series of splice-junction-specific primers and probes. The time courses of each HTLV-2 transcript in three different cellular systems, namely stably infected cells lines, transiently transfected cells and ex-vivo IL-2 stimulated PBMCs from infected subjects were investigated. The results obtained led to the quantitation of all known HTLV-2 mRNAs. Preliminary data showed different levels of env transcript in HTLV-2 subtypes A and B. Evidence for a differential env expression in HTLV-2B stably infected cells, prompted further investigation on the complex pattern of splicing between exons 1 and 2 and allowed the identification of a novel 3’ acceptor site (SS) of splicing. This novel 3’SS is used to express alternative spliced isoforms within the pX terminal region of HTLV-2, including the singly spliced env and the three doubly spliced bicistronic tax/rex, p10/p11 and 1-2-B transcripts. Results demonstrated that the novel 3’SS was utilised in both HTLV-2 subtypes, and that the novel env isoform, named env 1-2b, was preferentially expressed in 2B subtypes, while 2A subtypes used more efficiently the canonical splice site. The kinetics of total mRNA HTLV-2 expression in these three cellular systems presented a general pattern characterised by an initial low transcript level and a subsequent increase to reach a peak of expression after 21-24 hours in culture. The full length gag/pol mRNA was the most abundant one during the time course, and behaved as a late gene that peaked after 21 to 48 hours. The canonical env transcript was expressed at very low rates in stably infected cells, and it was undetectable in PBMCs from infected subjects and in cells transfected with the HTLV-2 proviral clone. By contrast, env 1-2b isoform was efficiently expressed in stably infected cells as well as in ex-vivo infected PBMCs, behaving as a late gene showing a gradual and steady increase in copy number and reaching maximum expression at 21 to 48 hours. The regulatory tax/rex gene was expressed early and with a high/intermediate transcription rate in HTLV-2B subtypes in both stably infected cells and ex-vivo PBMCs. In this study the kinetics of expression of the yet unkwnon 1-2-B gene was investigated and found to be expressed at high levels at early time points, whereas the doubly spliced mRNA of accessory p10/p11 genes were poorly expressed or under detection limit. Among the singly spliced mRNAs coding for other accessory proteins, the p28, p22/p20-II isoform was found to be highly expressed in both HTLV-2 A and B subtypes as compared to its alternative p28, p22/p20-I form. The APH-2 negative transcript was efficiently expressed at high levels in both stably infected and transfected cells and behaved as a late gene. However, in ex-vivo PBMCs its expression level and kinetics pattern appeared to be variable and a clear pattern of expression was not assessed. In conclusion, this study demonstrated that HTLV-2 transcripts of both A and B subtypes are differentially expressed. A temporal pattern of mRNA production, with early, tax/rex and 1-2-B and late, gag/pol, env, p28,p22/p20-II genes was established. The tax/rex early expression indicates that this protein is necessary at the beginning of the viral cycle to transactivate and regulate viral and cellular genes. Most structural genes were expressed late when the transcription of early genes was already decreasing, thus showing that a temporal switch was occurring between early to late genes production. This study also provided new clues on the selective use of alternative 3’SS within the pX region of HTLV-2 for both subtypes A and B. Overall these findings indicate that the control of HTLV-2 viral gene expression is highly regulated both in its kinetics and expression. Moreover, it suggests that the use of multiple acceptor sites might play an important role on the preferential expression of specific proteins in the different phases of the viral cycle.
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