Name: use of alu element containing minigenes to analyze circular rnas
Uploaded: 2020-03-10T12:00:00
Description: Watch this Scientific Journal Video about Use of Alu Element Containing Minigenes to Analyze Circular RNAs at JoVE.com

Questo lavoro è stato sostenuto dal Dipartimento della Difesa DoD grant A-180075. Stefan Stamm ringrazia Jacqueline Noonan Endowment. Anna Pawluchin è stata supportata dal DAAD, programma di scambio accademico tedesco, Justin R. Welden ha ricevuto il premio Max Steckler Award dell'Università del Kentucky.

1. Progettazione dei costrutti
<ol><li>Utilizzare il browser genoma UCSC24 per identificare gli elementi ripetitivi necessari per la formazione circolare di RNA e incorporarli nei costrutti. È importante sottolineare che i numeri di forza per l'amplificazione devono essere al di fuori degli elementi ripetitivi.</li>
	<li>Incollare la sequenza circolare dell'RNA (Supplemental Figure 1 è una sequenza di prova) in <a href="https://genome.ucsc.edu/cgi-bin/hgBlat?command=start" tar...

<ol>
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B., et al. <a target="_blank" href="http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=PubMed&cmd=Search&doptcmdl=Citation&defaultField=Title+Word&term=Natural+RNA+circles+function+as+efficient+microRNA+sponges.">Natural RNA circles function as efficient microRNA sponges.</a> Nature. 495 (7441), 384-388 (2013).</li><li>Kelly, S., Greenman, C., Cook, P. R., Papantonis, A. <a target="_blank" href="http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=PubMed&cmd=Search&doptcmdl=Citation&defaultField=Title+Word&term=Exon+Skipping+Is+Correlated+with+Exon+Circularization.">Exon Skipping Is Correlated with Exon Circularization.</a> Journal of Molecular Biology. 427 (15), 2414-2417 (2015).</li><li>Li, Z., et al. <a target="_blank" href="http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=PubMed&cmd=Search&doptcmdl=Citation&defaultField=Title+Word&term=Exon-intron+circular+RNAs+regulate+transcription+in+the+nucleus.">Exon-intron circular RNAs regulate transcription in the nucleus.</a> Nature Structural &amp; Molecular Biology. 22 (3), 256-264 (2015).</li><li>Yang, Y., et al. <a target="_blank" href="http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=PubMed&cmd=Search&doptcmdl=Citation&defaultField=Title+Word&term=Extensive+translation+of+circular+RNAs+driven+by+N(6)-methyladenosine.">Extensive translation of circular RNAs driven by N(6)-methyladenosine.</a> Cell Research. 27 (6), 626-641 (2017).</li><li>Abe, N., et al. <a target="_blank" href="http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=PubMed&cmd=Search&doptcmdl=Citation&defaultField=Title+Word&term=Rolling+Circle+Translation+of+Circular+RNA+in+Living+Human+Cells.">Rolling Circle Translation of Circular RNA in Living Human Cells.</a> Scientific Reports. 5, 16435 (2015).</li><li>Salzman, J., Chen, R. 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G., et al. <a target="_blank" href="http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=PubMed&cmd=Search&doptcmdl=Citation&defaultField=Title+Word&term=Enzymatic+assembly+of+DNA+molecules+up+to+several+hundred+kilobases.">Enzymatic assembly of DNA molecules up to several hundred kilobases.</a> Nature Methods. 6 (5), 343-345 (2009).</li><li>Conn, S. J., et al. <a target="_blank" href="http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=PubMed&cmd=Search&doptcmdl=Citation&defaultField=Title+Word&term=The+RNA+binding+protein+quaking+regulates+formation+of+circRNAs.">The RNA binding protein quaking regulates formation of circRNAs.</a> Cell. 160 (6), 1125-1134 (2015).</li><li>Jeck, W. R., Sharpless, N. 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C., et al. <a target="_blank" href="http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=PubMed&cmd=Search&doptcmdl=Citation&defaultField=Title+Word&term=Combinatorial+control+of+Drosophila+circular+RNA+expression+by+intronic+repeats,+hnRNPs,+and+SR+proteins.">Combinatorial control of Drosophila circular RNA expression by intronic repeats, hnRNPs, and SR proteins.</a> Genes &amp; Development. 29 (20), 2168-2182 (2015).</li><li>Starke, S., et al. <a target="_blank" href="http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=PubMed&cmd=Search&doptcmdl=Citation&defaultField=Title+Word&term=Exon+circularization+requires+canonical+splice+signals.">Exon circularization requires canonical splice signals.</a> Cell Reports. 10 (1), 103-111 (2015).</li><li>Suzuki, H., Tsukahara, T. <a target="_blank" href="http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=PubMed&cmd=Search&doptcmdl=Citation&defaultField=Title+Word&term=A+view+of+pre-mRNA+splicing+from+RNase+R+resistant+RNAs.">A view of pre-mRNA splicing from RNase R resistant RNAs.</a> International Journal of Molecular Sciences. 15 (6), 9331-9342 (2014).</li><li>Zhang, X. 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In generale, gli RNA circolari sono bassi abbondanti1, il che complica lo studio della loro funzione e formazione. Simile agli RNA lineari13, l'uso di minigeni reporter permette l'identificazione di cis e fattori trans-agire che regolano la formazione di RNA circolari. Pertanto, questo approccio genera ipotesi che possono essere ulteriormente testate utilizzando i geni endogeni.
Il passo più critico è la progettazione del gene reporter. L'assem...

RNA circolari Gli RNA circolari (circRNA) sono rna a singolo spiaggiamento chiusi covalentmente chiusi che sono espressi nella maggior parte degli organismi. Vengono generati unendo un sito di giunzione a un downstream 5' a un sito di giunzione a monte 3', un processo chiamato back-splicing (Figura 1A)1. Le sequenze nel pre-mRNA che presentano una base complementare fino a 30-40 nt portano i siti di giunzione posteriore in un corretto allineamento per la formazione di circRNA2. Nell'uomo, gli elementi Alu 1, che rappresentano circa l'11% del genoma3, formano ampie strutture di RNA a doppio filamento nel pre-mRNA a causa della loro auto-complementarità4,5 e quindi promuovono la formazione di circRNA1.
Attualmente, sono state descritte tre funzioni principali dei circRNA. Alcuni circRNA legano microRNA (miRNA) e attraverso il sequestro agiscono come spugne di miRNA6. I circRNA sono stati implicati nella regolazione trascrizionale e post trascrizionale, attraverso la concorrenza con la giunzione lineare7 o la modulazione dell'attività del fattore di trascrizione8. Infine, i circRNA contengono brevi cornici di lettura aperte e studi di prova di principio dimostrano che possono essere tradotti9,10. Tuttavia, la funzione della maggior parte dei circolrRNA rimane enigmatica. La maggior parte degli RNA circolari è stata rilevata utilizzando i metodi di sequenziamento di nuova generazione11. Analisi dettagliate di singoli geni utilizzando approcci RT-PCR mirati rivelano che un gran numero di RNA circolari rimane da scoprire12.
Uso dei geni dei reporter per analizzare l'elaborazione pre-mRNA L'analisi dell'mRNA derivato dai costrutti di segnalazione del DNA trasinfezione in cellule è un metodo ben consolidato per studiare lo splicing pre-mRNA alternativo, che può essere applicato agli RNA circolari. In generale, l'eson alternativo, gli introni circostanti e gli estrusioni coniugali vengono amplificati e clonati in un vettore di espressione eucatra. Spesso, gli introni sono accorciati. I costrutti sono trasfettati in cellule eucariotiche e di solito analizzati da RT-PCR13,14. Questo approccio è stato ampiamente utilizzato per mappare i siti di giunzione regolamentare e i fattori di trans-azione negli esperimenti di co-trasfezione13,15,16,17,18. Inoltre, la generazione di minigeni proteici ha permesso lo screening di sostanze che cambiano lo splicing alternativo19,20.
Il metodo è stato applicato agli RNA circolari. Attualmente, almeno 12 backbone minigene sono stati descritti nella letteratura e sono riassunti nella tabella 1. Ad eccezione del sistema di espressione basato sul tRNA21,22, tutti dipendono dai promotori di polimerasi II. Qui, descriviamo un metodo per generare minigeni di reporter umani per determinare i fattori di cis e trans-azione coinvolti nella generazione di RNA circolari. Una panoramica del metodo che utilizza sequenze di un reporter genepubblicato 23 è illustrata nella Figura 1.

<table border="1" fo:keep-together.within-page="1" fo:keep-with-next.within-page="always">
	<tbody>
		<tr>
			<td>(PEI) Hydrochloride</td>
			<td>Polysciences</td>
			<td>24765-1</td>
			<td></td>
		</tr>
		<tr>
			<td>Builder tool</td>
			<td>NEB</td>
			<td></td>
			<td><a href="https://nebuilder.neb.com/#!/" target="_blank">https://nebuilder.neb.com/#!/</a></td>
		</tr>
		<tr>
			<td>Dark Reader Transilluminator.</td>
			<td>Clare Chemical Research</td>
			<td></td>
			<td></td>
		</tr>
		<tr>
			<td>Enzymatic DNA assembly kit</td>
			<td>NEB</td>
			<td>E2621S</td>
			<td></td>
		</tr>
		<tr>
			<td>Gel and PCR cleanup kit</td>
			<td>Promega</td>
			<td>A9282</td>
			<td></td>
		</tr>
		<tr>
			<td>Glyco Blue</td>
			<td>Thermo Fisher</td>
			<td>AM9516</td>
			<td></td>
		</tr>
		<tr>
			<td>pcDNA3.1 cloning site</td>
			<td>Polycloning site</td>
			<td></td>
			<td><a href="https://assets.thermofisher.com/TFS-Assets/LSG/manuals/pcdna3_1_man.pdf" target="_blank">https://assets.thermofisher.com/TFS-Assets/LSG/manuals/pcdna3_1_man.pdf</a></td>
		</tr>
		<tr>
			<td>Polymerase 1</td>
			<td>NEB</td>
			<td>M0491L</td>
			<td>Q5 DNA polymerase</td>
		</tr>
		<tr>
			<td>Polymerase 2</td>
			<td>Biorad</td>
			<td>1725310</td>
			<td>Long range polymerase (NEB), iproof (BioRad)</td>
		</tr>
		<tr>
			<td>Polymerase 2</td>
			<td>Qiagen</td>
			<td>206402</td>
			<td>Qiagen long range polymerase kit</td>
		</tr>
		<tr>
			<td>Reverse Transcriptase</td>
			<td>Thermo Fisher</td>
			<td>18080044</td>
			<td></td>
		</tr>
		<tr>
			<td>RNA isolation kit</td>
			<td>Life Technologies</td>
			<td>12183025</td>
			<td>Ambion by Life Technologies</td>
		</tr>
		<tr>
			<td>RNAse R</td>
			<td>Lucigen</td>
			<td>RNR07250</td>
			<td>Epicenter/Lucigen</td>
		</tr>
		<tr>
			<td>Stable competent cells</td>
			<td>NEB</td>
			<td>C3040H</td>
			<td>NEB stable cells</td>
		</tr>
		<tr>
			<td>Standard cloning bacteria</td>
			<td>NEB</td>
			<td>C2988J</td>
			<td>NEB5-alpha competent</td>
		</tr>
		<tr>
			<td>Web tool to design primers</td>
			<td>NEB</td>
			<td></td>
			<td><a href="https://nebuilder.neb.com/#!/" target="_blank">https://nebuilder.neb.com/#!/</a></td>
		</tr>
		<tr>
			<td>Web-based temperature calculations</td>
			<td>NEB</td>
			<td></td>
			<td><a href="https://tmcalculator.neb.com/#!/main" target="_blank">https://tmcalculator.neb.com/#!/main</a></td>
		</tr>
	</tbody>
</table>

use of alu element containing minigenes to analyze circular rnas

Oltre agli mRNA lineari, molti geni eucarioti generano RNA circolari. La maggior parte degli RNA circolari sono generati dall'unendo un sito di giunzione di 5' con un sito di giunzione a monte a monte di 3' all'interno di un pre-mRNA, un processo chiamato back-splicing. Questa circolarizzazione è probabilmente aiutata da strutture secondarie nel pre-mRNA che portano i siti di giunzione in stretta vicinanza. Nei geni umani, si pensa che gli elementi alu promuovano queste strutture secondarie dell'RNA, poiché gli elementi Alu sono abbondanti e presentano complementarità di base tra loro quando sono presenti in direzioni opposte nel pre-mRNA. Qui, descriviamo la generazione e l'analisi di grandi elementi Alu contenenti geni reporter che formano RNA circolari. Attraverso l'ottimizzazione dei protocolli di clonazione, è possibile generare geni reporter con una lunghezza di inserto fino a 20 kb. La loro analisi negli esperimenti di co-trasfezione consente l'identificazione di fattori normativi. Pertanto, questo metodo può identificare le sequenze di RNA e i componenti cellulari coinvolti nella formazione circolare dell'RNA.

I geni dei reporter consentono la determinazione di fattori regolatori che influenzano la formazione circolare dell'RNA. Tuttavia, questi geni reporter sono grandi e contengono elementi ripetitivi che spesso rendono instabili i costrutti del DNA. A causa delle loro grandi dimensioni, è spesso necessario eliminare parti degli introni, che si ottiene amplificando i pezzi genomici contenenti gli esoni e le parti intronica laterali più piccole. Questi pezzi di DNA sono assemblati enzimaticamente, permettendo la costruzione...

Watch this Scientific Journal Video about Use of Alu Element Containing Minigenes to Analyze Circular RNAs at JoVE.com

Use of Alu Element Containing Minigenes to Analyze Circular RNAs

Cloniamo e analizziamo i geni dei reporter generando RNA circolari. Questi geni reporter sono più grandi dei costrutti per analizzare lo splicing lineare e contenere elementi Alu. Per studiare gli RNA circolari, i costrutti vengono trasfettati in cellule e l'RNA risultante viene analizzato utilizzando RT-PCR dopo la rimozione dell'RNA lineare.

Uso dell'elemento Alu contenente Minigenes per analizzare gli RNA circolari

In addition to linear mRNAs, many eukaryotic genes generate circular RNAs. Most circular RNAs are generated by joining a 5&#39; splice site with an ...

Questo protocollo è significativo perché consente all'utente di generare un sistema di espressione genomica che può subire splicing alternativo e in questo caso formare RNA circolari che possono essere testate per la loro funzione e associazione di malattie. Il vantaggio principale di questa tecnica è che aprirà la strada ad altri per utilizzare questo protocollo in biologia molecolare e clonazione quando studiano lo splicing alternativo nella formazione e nella funzione dell'RNA circolare. Il mio consiglio a qualcuno che prova questa tecnica per la prima volta sarebbe quello di ottimizzare le condizioni PCR.Eseguire gradienti o eseguire touchdown PCR con diverse temperature di ricottura e tempi di estensione. Di solito frammenti più lunghi superiori a sei KB estenderanno un KB per ciclo e diverse temperature di ricottura dovrebbero essere testate per la migliore amplificazione. La dimostrazione di questo metodo è fondamentale perché darà agli utenti una migliore rappresentazione visiva degli aspetti più difficili della procedura, in particolare la generazione di primer.Per iniziare questa procedura, caricare il browser del genoma UCSC e utilizzarlo per identificare gli elementi ripetitivi necessari per la formazione di RNA circolari e incorporarli nei costrutti. È importante sottolineare che i primer per l'amplificazione devono essere al di fuori degli elementi ripetitivi. Incollare la sequenza di RNA circolare nella ricerca blat umana e selezionare l'organismo giusto.Invia la sequenza, vai alla visualizzazione del browser e ingrandisci 1,5 timer o, a caso. Quindi, passare il mouse sugli elementi ripetitivi per identificarne il sottotipo in una finestra mobile. Gli elementi Alu sono nella linea del seno.Utilizzare il pulsante traccia predefinito sotto la finestra per reimpostare il browser se si ottiene un'immagine errata. Per prima cosa vai a vedere, DNA sulla linea superiore del browser del genoma USCS per scaricare la sequenza di DNA mostrata nella finestra. Nell'opzione di formattazione sequenziamento selezionare le opzioni estese maiuscole/minuscole/colore.Selezionate il caso di default come inferiore e selezionate attiva/disattiva maiuscole/minuscole per NCBI RefSeq. Selezionate sottolineatura e grassetto (Bold) e Corsivo (Italic) per RepeatMasker. Fare clic su Invia.Ci saranno esoni come lettere maiuscole e introni come lettere minuscole. Controllare i bordi dell'esone/introne. Se il browser mostra il complemento inverso, tornare indietro e selezionare la casella del complemento inverso fino a visualizzare i bordi esone/introne corretti.Copiare quindi il file con l'orientamento corretto in un documento di elaborazione testi ed evidenziare gli esoni. Selezionate i frammenti da amplificare assicurandoche l'introne non inizi o finisca in una regione ripetitiva poiché i primer in queste regioni non amplificano sequenze specifiche. Per iniziare, usa uno strumento Web per progettare i primer per la clonazione.Per la sequenza vettoriale, aggiungere il sito di inserimento come ultimo nucleotide e successivamente aggiungere i frammenti. Poiché la numerazione vettoriale non inizia con un dato sito di inserimento, il sito di inserimento nel vettore si trova e la parte downstream viene messa davanti alla sequenza a monte. Regolare i primer se i loro punti di fusione sono distanti più di quattro gradi Celsius e non funzionano nell'amplificazione.In questo studio, i geni reporter che generano RNA circolari vengono clonati e analizzati. I prodotti PCR ottimizzati sono separati su un gel di agarosio dell'1% contenente gel verde 1X. Le singole bande rappresentano i prodotti PCR che verranno utilizzati nell'assemblaggio del DNA enzimatico.Queste bande vengono quindi tagliate dal gel e purificate. Il prodotto PCR purificato non è fedele alle dimensioni previste con gel verde, quindi i prodotti sono separati anche su un gel di agarosio all'1% che viene successivamente colorato con bromuro di etidio per garantire che i prodotti siano delle dimensioni corrette. Per iniziare, impostare un kit di assemblaggio enzimatico del DNA.Combinare il vettore e gli inserti in un rapporto molare da uno a due. Quindi, aggiungere 10 microlitri di mix master di assemblaggio del DNA. Incubare i campioni per 60 minuti a 50 gradi.Scongelare le cellule competenti sul ghiaccio durante l'incubazione. Le cellule devono essere in un volume di 50 microlitri. Quindi, trasformare le cellule competenti con la reazione totale di assemblaggio.Aggiungere due microlitri del prodotto assemblato refrigerato alle celle competenti. Mescolare facendo scorrere delicatamente il tubo da quattro a cinque volte. Non vortice.Mettere la miscela sul ghiaccio per 30 minuti. Scaldare la miscela a 42 gradi Celsius per 30 secondi. Quindi riposizionare sul ghiaccio per due minuti.Successivamente, aggiungere 950 microlitri di supporti SOC a temperatura ambiente al tubo. Incubare a 37 gradi Celsius per 60 minuti mentre si trema a 300 giri/min. Durante questa incubazione, riscaldare due piastre di selezione che contengono l'antibiotico appropriato.Dopo l'incubazione, centrifugare il tubo di reazione a 10.000 g per 30 secondi per pellettare le cellule e placcare il 25% delle cellule su una piastra di selezione e il 75% dall'altra. Incubare queste piastre durante la notte a 37 gradi Celsius. Prima di iniziare la trasfezione, controllare il DNA per restrizione digerire.Qui, un tau minigene rappresentativo che contiene esoni da nove a 12 viene tagliato con enzimi di restrizione indicati per escludere le principali ricombinazioni. Per la trasfezione, sciogliere prima il cloridrato lineare di polietilene in acqua ad una concentrazione di un milligrammo per millilitro a pH due. Utilizzare idrossido di sodio per portare il pH fino a sette e filtrare sterilemente la soluzione con un filtro da 0,22 micrometri.Conservare la soluzione a quattro gradi Celsius fino a quando non è pronta per l'uso. Quindi dividere le cellule nei pozzi di una piastra a sei porri e lasciarle crescere durante la notte su supporti DMEM contenenti il 10% fbs. Il giorno dopo, aliquote un microgrammo del gene riportato in un tubo sterile e aggiungere 200 microlitri di cloruro di sodio filtrato sterile da 150 millimolare.Mescolare con il vortice. Successivamente, aggiungere la soluzione di polietilenimina a questa miscela con un rapporto di tre microlitri di polietilenimina per ogni microgrammo di DNA. Centrifugare brevemente per raccogliere campioni nella parte inferiore del tubo.Incubare i campioni a temperatura ambiente per 10 minuti. Quindi aggiungerlo direttamente alle celle HEK293. Incubare le cellule durante la notte a 37 gradi Celsius con il 5% di anidride carbonica.Il giorno dopo, usa un kit di isolamento dell'RNA per isolare l'RNA per RT-PCR. cDNA da due campioni derivati da tessuti cerebrali umani sono amplificati con primer circolari di RNA che circondano l'esone 1210 inverso e l'esone circolare 1211 in avanti. Mentre si vede la banda prevista corrispondente all'RNA circolare tau, le altre bande forti sono artefatti che non corrispondevano al genoma umano.Questo esperimento viene ripetuto con identiche condizioni PCR, ma la trascrizione inversa è stata eseguita solo con il primer inverso circ tau exon 1210. Solo la banda prevista viene amplificata e convalidata tramite sequenziamento. L'RNA viene quindi trattato con RNasi R che rimuove l'RNA lineare.L'RNA circolare è rilevabile dopo il trattamento mentre l'RNA lineare non fornisce più un segnale rilevabile. L'RNA è isolato 24 ore dopo la trasfezione e analizzato da RT-PCR. L'amplificazione dell'mRNA tau lineare mostra due bande dovute allo splicing alternativo dell'esone 10.Il loro rapporto cambia con l'espressione over dei fattori di splicing. L'amplificazione dell'RNA tau circolare 1210 mostra la dipendenza dell'espressione dell'RNA tau circ sull'espressione di alcuni fattori di giunzione in particolare la chinasi CLK2 simile alla Cdc2 e la proteina SR 9G8. La cosa più importante da ricordare quando si tenta questa procedura è la progettazione e la posizione dei primer quando si costruisce un minigene.Il primer non dovrebbe trovarsi in elementi ripetitivi e dovrà essere ottimizzato in condizioni diverse a seconda del frammento amplificato. Seguendo questa procedura, altri metodi che possono essere eseguiti testeranno la funzione degli RNA circolari. Gli utenti possono testare la traduzione o il sequestro delle proteine per identificare una funzione per lo specifico RNA circolare a cui l'utente è interessato.Questa tecnica ha spianato la strada all'utilizzo di frammenti genomici in un sistema minigene in grado di esprimere es oltre gli RNA circolari consentendo all'utente di testare e identificare la propria funzione e in alcuni aspetti la loro associazione alla malattia. L'implicazione di questa tecnica si estende verso potenziali terapie e diagnostica di una particolare malattia, ad esempio tauopatie, malattie neurodegenerative associate alla patologia tau. Abbiamo scoperto che la proteina tau associata ai microtubuli, nota come MAPT, genera RNA circolari che crediamo contribuiscano alla patologia della malattia e questo metodo ci consente di studiare completamente questi RNA circolari e identificarne la funzione e la relazione con la malattia.Questo metodo potrebbe fornire informazioni su una migliore comprensione degli RNA circolari, delle loro funzioni e del ruolo che possono svolgere in determinate malattie. Questo metodo può essere applicato nella clonazione di altri minigeni che esprimono RTA circolari tra le specie in cui può fornire informazioni sulla loro funzione. L'amplificazione dei prodotti PCR si rivela la più difficile con lunghi frammenti amplificati dal DNA genomico, insieme ad avere più elementi ripetitivi all'interno del frammento.

use-of-alu-element-containing-minigenes-to-analyze-circular-rnas

Research

JoVE Journal

Biochemistry

Use of Alu Element Containing Minigenes to Analyze Circular RNAs

Combining Wet and Dry Lab Techniques to Guide the Crystallization of Large Coiled-coil Containing Proteins

Obtaining crystals for structure determination can be a difficult and time consuming proposition for any protein. Coiled-coil proteins and domains are found throughout nature, however, because of their physical properties and tendency to aggregate, they are traditionally viewed as being especially difficult to crystallize. Here, we utilize a variety of quick and simple techniques designed to identify a series of possible domain boundaries for a given coiled-coil protein, and then quickly characterize the behavior of these proteins in solution. With the addition of a strongly fluorescent tag (mRuby2), protein characterization is simple and straightforward. The target protein can be readily visualized under normal lighting and can be quantified with the use of an appropriate imager. The goal is to quickly identify candidates that can be removed from the crystallization pipeline because they are unlikely to succeed, affording more time for the best candidates and fewer funds expended on proteins that do not produce crystals. This process can be iterated to incorporate information gained from initial screening efforts, can be adapted for high-throughput expression and purification procedures, and is augmented by robotic screening for crystallization.

We describe a framework incorporating straightforward biochemical and computational analysis to guide the characterization and crystallization of large coiled-coil domains. This framework can be adapted for globular proteins or extended to incorporate a variety of high-throughput techniques.

La combinazione di Wet and Dry tecniche di laboratorio per guidare la cristallizzazione di grandi dimensioni avvolto a spirale contenenti proteine

Obtaining crystals for structure determination can be a difficult and time consuming proposition for any protein. Coiled-coil proteins and domains are ...

Ricerca

Biochimica

Method to Visualize and Analyze Membrane Interacting Proteins by Transmission Electron Microscopy

Monotopic proteins exert their function when attached to a membrane surface, and such interactions depend on the specific lipid composition and on the availability of enough area to perform the function. Nanodiscs are used to provide a membrane surface of controlled size and lipid content. In the absence of bound extrinsic proteins, sodium phosphotungstate-stained nanodiscs appear as stacks of coins when viewed from the side by transmission electron microscopy (TEM). This protocol is therefore designed to intentionally promote stacking; consequently, the prevention of stacking can be interpreted as the binding of the membrane-binding protein to the nanodisc. In a further step, the TEM images of the protein-nanodisc complexes can be processed with standard single-particle methods to yield low-resolution structures as a basis for higher resolution cryoEM work. Furthermore, the nanodiscs provide samples suitable for either TEM or non-denaturing gel electrophoresis. To illustrate the method, Ca2+-induced binding of 5-lipoxygenase on nanodiscs is presented.

Many proteins perform their function when attached to membrane surfaces. The binding of extrinsic proteins on nanodisc membranes can be indirectly imaged by transmission electron microscopy. We show that the characteristic stacking (rouleau) of nanodiscs induced by the negative stain sodium phosphotungstate is prevented by the binding of extrinsic protein.

Metodo per visualizzare e analizzare membrana proteine ​​interagenti con microscopia elettronica a trasmissione

Monotopic proteins exert their function when attached to a membrane surface, and such interactions depend on the specific lipid composition and on the ...

Quantification of the Abundance and Charging Levels of Transfer RNAs in Escherichia coli

Transfer RNA (tRNA) is an essential part of the translational machinery in any organism. tRNAs bind and transfer amino acids to the translating ribosome. The relative levels of different tRNAs, and the ratio of aminoacylated tRNA to total tRNA, known as the charging level, are important factors in determining the accuracy and speed of translation. Therefore, the abundance and charging levels of tRNAs are important variables to measure when studying protein synthesis, for example under various stress conditions. Here, we describe a method for harvesting tRNA and directly measuring both the relative abundance and the absolute charging level of specific tRNA species in Escherichia coli. The tRNA is harvested in such a way that the labile bond between the tRNA and its amino acid is preserved. The RNA is then subjected to gel electrophoresis and Northern blotting, which results in separation of the charged and uncharged tRNAs. The levels of specific tRNAs in different samples can be compared due to the addition of spike-in cells for normalization. Prior to RNA purification, we add 5% of E. coli cells that overproduce the rare tRNAselC to each sample. The amount of the tRNA species of interest in a sample is then normalized to the amount of tRNAselC in the same sample. Addition of spike-in cells prior to RNA purification has the advantage over addition of purified spike-in RNAs that it also accounts for any differences in cell lysis efficiency between samples.

Quantification of the Abundance and Charging Levels of Transfer RNAs in Escherichia coli

Here we present a method for directly measuring transfer RNA charging levels from purified Escherichia coli RNA as well as a way to compare relative levels of transfer RNA, or any other short RNA, across different samples based on the addition of spike-in cells expressing a reference gene.

Quantificazione di abbondanza e ricarica i livelli di RNA di trasferimento in Escherichia coli

Transfer RNA (tRNA) is an essential part of the translational machinery in any organism. tRNAs bind and transfer amino acids to the translating ribosome. ...

Simultaneous Measurement of Superoxide/Hydrogen Peroxide and NADH Production by Flavin-containing Mitochondrial Dehydrogenases

It has been reported that mitochondria can contain up to 12 enzymatic sources of reactive oxygen species (ROS). A majority of these sites include flavin-dependent respiratory complexes and dehydrogenases that produce a mixture of superoxide (O2&#9679;-) and hydrogen peroxide (H2O2). Accurate quantification of the ROS-producing potential of individual sites in isolated mitochondria can be challenging due to the presence of antioxidant defense systems&#160;and side reactions that also form O2&#9679;-/H2O2. Use&#160;of nonspecific inhibitors that can disrupt mitochondrial bioenergetics can also compromise measurements by altering&#160;ROS release from other sites of production. Here, we present an easy method for the simultaneous measurement of H2O2 release and nicotinamide adenine dinucleotide (NADH) production by purified flavin-linked dehydrogenases. For our purposes here, we have used purified pyruvate dehydrogenase complex (PDHC) and &#945;-ketoglutarate dehydrogenase complex (KGDHC) of porcine heart origin as examples. This method allows for an accurate measure of native H2O2 release rates by individual sites of production by eliminating other potential sources of ROS and antioxidant systems. In addition, this method allows for a direct comparison of the relationship between H2O2 release and enzyme activity and the screening of the effectiveness and selectivity of inhibitors for ROS production. Overall, this approach can allow for the in-depth assessment of native rates of ROS release for individual enzymes prior to conducting more sophisticated experiments with isolated mitochondria or permeabilized muscle fiber.

Mitochondria contain several flavin-dependent enzymes that can produce reactive oxygen species (ROS). Monitoring ROS release from individual sites in mitochondria is challenging due to unwanted side reactions. We present an easy, inexpensive method for direct assessment of native rates for ROS release using purified flavoenzymes and microplate fluorometry.

Misura simultanea di perossido di idrogeno/del superossido e produzione di NADH di Flavin-contenente deidrogenasi mitocondriale

It has been reported that mitochondria can contain up to 12 enzymatic sources of reactive oxygen species (ROS). A majority of these sites include ...

Use of Two Dimensional Semi-denaturing Detergent Agarose Gel Electrophoresis to Confirm Size Heterogeneity of Amyloid or Amyloid-like Fibers

Amyloid or amyloid-like fibers have been associated with many human diseases, and are now being discovered to be important for many signaling pathways. The ability to readily detect the formation of these fibers under various experimental conditions is essential for understanding their potential function. Many methods have been used to detect the fibers, but not without some drawbacks. For example, electron microscopy (EM), or staining with Congo Red or Thioflavin T often requires purification of the fibers. On the other hand, semi-denaturing detergent agarose gel electrophoresis (SDD-AGE) allows detection of the SDS-resistant amyloid-like fibers in the cell extracts without purification. In addition, it allows the comparison of the size difference of the fibers. More importantly, it can be used to identify specific proteins within the fibers by Western blotting. It is less time consuming and more easily accessible to a wider number of labs. SDD-AGE results often show variable degree of heterogeneity. It raises the question whether part of the heterogeneity results from the dissociation of the protein complex during the electrophoresis in the presence of SDS. For this reason, we have employed a second dimension of SDD-AGE to determine if the size heterogeneity seen in SDD-AGE is truly a result of fiber heterogeneity in vivo and not a result of either degradation or dissociation of some of the proteins during electrophoresis. This method allows fast, qualitative confirmation that the amyloid or amyloid-like fibers are not partially dissociating during the SDD-AGE process.

Here we use two-dimensional semi-denaturing agarose gel electrophoresis to confirm the presence of amyloid-like fibers of heterogeneous size and exclude the possibility that the size heterogeneity is due to dissociation of the amyloid fibers during the gel running process.

Uso di elettroforesi del Gel di agarosio detergente semi-denaturante dimensionale due per confermare dimensioni eterogeneità delle fibre amiloidi o amiloide-come

Amyloid or amyloid-like fibers have been associated with many human diseases, and are now being discovered to be important for many signaling pathways. ...

Large-scale Production of Recombinant RNAs on a Circular Scaffold Using a Viroid-derived System in Escherichia coli

With increasing interest in RNA biology and the use of RNA molecules in sophisticated biotechnological applications, the methods to produce large amounts of recombinant RNAs are limited. Here, we describe a protocol to produce large amounts of recombinant RNA in Escherichia coli based on co-expression of a chimeric molecule that contains the RNA of interest in a viroid scaffold and a plant tRNA ligase. Viroids are relatively small, non-coding, highly base-paired circular RNAs that are infectious to higher plants. The host plant tRNA ligase is an enzyme recruited by viroids that belong to the family Avsunviroidae, such as Eggplant latent viroid (ELVd), to mediate RNA circularization during viroid replication. Although ELVd does not replicate in E. coli, an ELVd precursor is efficiently transcribed by the E. coli RNA polymerase and processed by the embedded hammerhead ribozymes in bacterial cells, and the resulting monomers are circularized by the co-expressed tRNA ligase reaching a remarkable concentration. The insertion of an RNA of interest into the ELVd scaffold enables the production of tens of milligrams of the recombinant RNA per liter of bacterial culture in regular laboratory conditions. A main fraction of the RNA product is circular, a feature that facilitates the purification of the recombinant RNA to virtual homogeneity. In this protocol, a complementary DNA (cDNA) corresponding to the RNA of interest is inserted in a particular position of the ELVd cDNA in an expression plasmid that is used, along the plasmid to co-express eggplant tRNA ligase, to transform E. coli. Co-expression of both molecules under the control of strong constitutive promoters leads to production of large amounts of the recombinant RNA. The recombinant RNA can be extracted from the bacterial cells and separated from the bulk of bacterial RNAs taking advantage of its circularity.

Large-scale Production of Recombinant RNAs on a Circular Scaffold Using a Viroid-derived System in Escherichia coli

Here, we present a protocol to produce large amounts of recombinant RNA in Escherichia coli by co-expressing a chimeric RNA that contains the RNA of interest in a viroid scaffold and a plant tRNA ligase. The main product is a circular molecule that facilitates purification to homogeneity.

Produzione su larga scala di RNA ricombinante su un'impalcatura circolare utilizzando un sistema derivato Viroid in Escherichia coli

With increasing interest in RNA biology and the use of RNA molecules in sophisticated biotechnological applications, the methods to produce large amounts ...

Expression, Purification, Crystallization, and Enzyme Assays of Fumarylacetoacetate Hydrolase Domain-Containing Proteins

Fumarylacetoacetate hydrolase (FAH) domain-containing proteins (FAHD) are identified members of the FAH superfamily in eukaryotes. Enzymes of this superfamily generally display multi-functionality, involving mainly hydrolase and decarboxylase mechanisms. This article presents a series of consecutive methods for the expression and purification of FAHD proteins, mainly FAHD protein 1 (FAHD1) orthologues among species (human, mouse, nematodes, plants, etc.). Covered methods are protein expression in E. coli, affinity chromatography, ion exchange chromatography, preparative and analytical gel filtration, crystallization, X-ray diffraction, and photometric assays. Concentrated protein of high levels of purity (&#62;98%) may be employed for crystallization or antibody production. Proteins of similar or lower quality may be employed in enzyme assays or used as antigens in detection systems (Western-Blot, ELISA). In the discussion of this work, the identified enzymatic mechanisms of FAHD1 are outlined to describe its hydrolase and decarboxylase bi-functionality in more detail.

Expression and purification of fumarylacetoacetate hydrolase domain-containing proteins is described with examples (expression in E. coli, FPLC). Purified proteins are used for crystallization and antibody production and employed for enzyme assays. Selected photometric assays are presented to display the multi-functionality of FAHD1 as oxaloacetate decarboxylase and acylpyruvate hydrolase.

Espressione, purificazione, cristallizzazione e saggi enzimatici di Fumarylacetoacetate Hydrolase Domain-Containing Proteins

Fumarylacetoacetate hydrolase (FAH) domain-containing proteins (FAHD) are identified members of the FAH superfamily in eukaryotes. Enzymes of this ...

Use of Microscale Thermophoresis to Measure Protein-Lipid Interactions

The ability to determine the binding affinity of lipids to proteins is an essential part of understanding protein-lipid interactions in membrane trafficking, signal transduction and cytoskeletal remodeling. Classic tools for measuring such interactions include surface plasmon resonance (SPR) and isothermal titration calorimetry (ITC). While powerful tools, these approaches have setbacks. ITC requires large amounts of purified protein as well as lipids, which can be costly and difficult to produce. Furthermore, ITC as well as SPR are very time consuming, which could add significantly to the cost of performing these experiments. One way to bypass these restrictions is to use the relatively new technique of microscale thermophoresis (MST). MST is fast and cost effective using small amounts of sample to obtain a saturation curve for a given binding event. There currently are two types of MST systems available. One type of MST requires labeling with a fluorophore in the blue or red spectrum. The second system relies on the intrinsic fluorescence of aromatic amino acids in the UV range. Both systems detect the movement of molecules in response to localized induction of heat from an infrared laser. Each approach has its advantages and disadvantages. Label-free MST can use untagged native proteins; however, many analytes, including pharmaceuticals, fluoresce in the UV range, which can interfere with determination of accurate KD values. In comparison, labeled MST allows for a greater diversity of measurable pairwise interactions utilizing fluorescently labeled probes attached to ligands with measurable absorbances in the visible range as opposed to UV, limiting the potential for interfering signals from analytes.

Microscale thermophoresis obtains binding constants quickly at low material cost. Either labeled or label free microscale thermophoresis is commercially available; however, label free thermophoresis is not capable of the diversity of interaction measurements that can be performed using fluorescent labels. We provide a protocol for labeled thermophoresis measurements.

Uso della termoforesi su microscala per misurare le interazioni proteina-lipidi

The ability to determine the binding affinity of lipids to proteins is an essential part of understanding protein-lipid interactions in membrane ...

Ready-To-Use qPCR for Detection of DNA from Trypanosoma cruzi or Other Pathogenic Organisms

Real-time PCR (qPCR) is a remarkably sensitive and precise technique&#160;that allows for amplifying&#160;minute amounts of nucleic acid targets from a multitude of samples. It has been extensively used in many research areas and achieved industrial application in fields such as human diagnostics and trait selection in crops of genetically modified organisms (GMO) crops. However, qPCR is not an error-proof technique. Mixing all reagents into a single master mix subsequently distributed onto 96 wells of a regular qPCR plate might lead to operator mistakes such as incorrect mixing of reagents or inaccurate dispensing into the wells. Here, a technique called gelification is presented, whereby most of the water present in the master mix is substituted by reagents that form a sol-gel mixture when submitted to a vacuum. As a result, qPCR reagents are effectively preserved for a few weeks at room temperature or a few months at 2-8 oC. Details of preparing each solution are shown here along with the expected aspect of a gelified reaction designed to detect&#160;T. cruzi satellite DNA (satDNA). A similar procedure can be applied to detect other organisms. Starting a gelified qPCR run is as simple as removing the plate from the refrigerator, adding the samples to their respective wells, and starting the run, thus decreasing the setup time of a full-plate reaction to the time it takes to load the samples. Additionally, gelified PCR reactions can be produced and controlled for quality in batches, saving time and avoiding common operator mistakes while running routine PCR reactions.

Ready-To-Use qPCR for Detection of DNA from Trypanosoma cruzi or Other Pathogenic Organisms

The present work describes the steps for producing ready-to-use qPCR for T. cruzi DNA detection that can be pre-loaded on the reaction vessel and stored in the refrigerator for several months.

qPCR pronta all'uso per la rilevazione del DNA da Trypanosoma cruzi o altri organismi patogeni

Real-time PCR (qPCR) is a remarkably sensitive and precise technique&#160;that allows for amplifying&#160;minute amounts of nucleic acid targets from a ...

Formulation and Characterization of Bioactive Agent Containing Nanodisks

The term nanodisk refers to a discrete type of nanoparticle comprised of a bilayer forming lipid, a scaffold protein, and an integrated bioactive agent. Nanodisks are organized as a disk-shaped lipid bilayer whose perimeter is circumscribed by the scaffold protein, usually a member of the exchangeable apolipoprotein family. Numerous hydrophobic bioactive agents have been efficiently solubilized in nanodisks by their integration into the hydrophobic milieu of the particle&#39;s lipid bilayer, yielding a largely homogenous population of particles in the range of 10-20 nm in diameter. The formulation of nanodisks requires a precise ratio of individual components, an appropriate sequential addition of each component, followed by bath sonication of the formulation mixture. The amphipathic scaffold protein spontaneously contacts and reorganizes the dispersed bilayer forming lipid/bioactive agent mixture to form a discrete, homogeneous population of nanodisk&#160;particles. During this process, the reaction mixture transitions from an opaque, turbid appearance to a clarified sample that, when fully optimized, yields no precipitate upon centrifugation. Characterization studies involve the determination of bioactive agent solubilization efficiency, electron microscopy, gel filtration chromatography, ultraviolet visible (UV/Vis) absorbance spectroscopy, and/or fluorescence spectroscopy. This is normally followed by an investigation of biological activity using cultured cells or mice. In the case of nanodisks harboring an antibiotic (i.e., the macrolide polyene antibiotic amphotericin B), their ability to inhibit the growth of yeast or fungi as a function of concentration or time can be measured. The relative ease of formulation, versatility with respect to component parts, nanoscale particle size, inherent stability, and aqueous solubility permits myriad in vitro and in vivo applications of nanodisk technology. In the present article, we describe a general methodology to formulate and characterize nanodisks containing amphotericin&#160;B as the hydrophobic bioactive agent.

Here, we describe the production and characterization of bioactive agents containing nanodisks. Amphotericin B nanodisks are taken as an example to describe the protocol in a stepwise manner.

Formulazione e caratterizzazione di agenti bioattivi contenenti nanodischi

The term nanodisk refers to a discrete type of nanoparticle comprised of a bilayer forming lipid, a scaffold protein, and an integrated bioactive agent. ...