post-transcriptional methylation removal in rnas using alkb demethylase and subsequent rna-cdna hybrid hydrolysis in rna sequencing preparation

Analisi della dinamica del tRNA con AQRNA-seq

Next-generation sequencing (NGS), also known as massively parallel sequencing, is a DNA sequencing technology that involves DNA fragmentation, ligation of adaptor oligonucleotides, polymerase chain reaction (PCR)-based amplification, sequencing of the DNA, and reassembly of the fragment sequences into a genome. The adaptation of NGS to sequence RNA (RNA-seq) is a powerful approach to identify and quantify RNA transcripts and their variants1. Innovative developments in RNA library preparation workflows and bioinformatic analysis pipelines, coupled with advancements in laboratory instrumentation, have expanded the repertoire of RNA-seq applications, progressing beyond exome sequencing into advanced functional omics like non-coding RNA profiling2, single cell analysis3, spatial transcriptomics4,5, alternative splicing analysis6, among others. These advanced RNA-seq methods reveal complex RNA functions through quantitative analysis of the transcriptome in normal and diseased cells and tissue.
Despite these advances in RNA-seq, several key technical features limit the quantitative power of the method. While most RNA-seq methods allow precise and accurate quantification of changes in the levels of RNAs between experimental variables (i.e., biological samples and/or physiological states), they cannot provide quantitative comparisons of the levels of RNA molecules within a sample. For example, most RNA-seq methods cannot accurately quantify the relative number of copies of individual tRNA isoacceptor molecules in a cellular pool of expressed tRNAs. As highlighted in the companion publication7, this limitation to RNA-seq arises from several features of RNA structure and the biochemistry of library preparation. For example, the activity of the ligation enzymes used to attach the 3&#39;- and 5&#39;-end sequencing linkers to RNA molecules is strongly influenced by the identity of the terminal nucleotides of the RNA and the sequencing linkers. This leads to large variations in efficiencies of linker ligations and profound artifactual increases in sequencing reads8,9,10.
A second set of limitations arise from the inherent structural properties of RNA molecules. Specifically, RNA secondary structure formation and dynamic changes in the dozens of post-transcriptional RNA modifications of the epitranscriptome&#160;can cause polymerase fall-off or mutation during reverse transcription. These errors result in incomplete or truncated cDNA synthesis or altered RNA sequence. While both of these phenomena can be exploited to map secondary structures or some modifications, they degrade the quantitative accuracy of RNA-seq if subsequent library preparation steps fail to capture truncated cDNAs or if data processing throws out mutated sequences not matching a reference dataset11,12. Furthermore, the immense chemical, length, and structural diversity of RNA transcripts, as well as the lack of tools to uniformly fragment long RNAs, diminishes the applicability of most RNA-seq methods to all RNA species13.
The AQRNA-seq (absolute quantification RNA sequencing) method has been developed to remove several of these technical and biological constraints that limit quantitative accuracy7. By minimizing sequence-dependent biases in capture, ligation, and amplification during RNA sequencing library preparation, AQRNA-seq achieves superior linearity compared to other methods, accurately quantifying 75% of a reference library of 963 miRNAs within 2-fold accuracy. This linear correlation of sequencing read count and RNA abundance is also observed in an analysis of a variable length pool of RNA oligonucleotide standards and in reference to orthogonal methods like northern blotting. Establishing linearity between sequencing read count and RNA abundance enables AQRNA-seq to achieve accurate, absolute quantification of all RNA species within a sample.
Here is a description of the protocol for AQRNA-seq library preparation workflow and the accompanying downstream data analytics pipeline. The method was applied to elucidate the dynamics of tRNA abundance during starvation-induced dormancy and subsequent resuscitation in&#160;the Mycobacterium bovis bacilli de Calmette et Gu&#233;rin (BCG) model of tuberculosis. Results were presented for the exploratory visualization of the sequencing data, along with subsequent clustering and differential expression analyses that unveiled discernable patterns in tRNA abundance associated with various phenotypes.

Autore in primo piano: Ruolo di AQRNA-seq nella mappatura di piccoli RNA e nel disfacimento dei meccanismi di traduzione delle proteine

AQRNA-seq per la quantificazione di piccoli RNA

AQRNA sequencing quantitatively maps small RNAs such as microRNAs, tRNAs, and tRNA fragments in virtually any cell or tissue sample. It can be used to map some of the 170 known tRNA modifications, but there are other methods that are more specific for mapping. You can use AQRNA-seq to discover disease biomarkers in the RNome and explore protein translation mechanisms at the systems level.Most RNA-seq methods can't accurately quantify the abundance of individual RNA molecules in a sample. This is caused by both structural properties of the RNA, such as secondary structures, post transcriptional modifications, as well as the biochemistry of library preparation such as ligation biases of a thousand fold induced by the terminal nucleotides on the RNAs. AQRNA-seq was developed to overcome several technical and biological challenges, limiting the accurate quantification of RNA abundance in the sample.Compared to other matters, it achieves linearity between recounts and copy numbers of RNA molecules, accurately, it quantifies 75%of a reference library, compressing 963 microRNAs with twofold accuracy. AQRNA-seq is unique in providing absolute quantification of small RNAs. This links the sequencing recounts directly to the number of copies of an RNA molecule in the sample.This level of accuracy is crucial for comparing dozens to hundreds of tRNAs in a sample, and it's unlike regular small RNA-seq, which only permits relative quantification across conditions and samples. We designed AQRNA-seq for an unmet need in understanding protein translation. We found that cells reprogrammed dozens of tRNA modifications in the number of copies of the modified tRNAs, to allow selective translation of messenger RNAs that are enriched with codons matching those tRNAs.AQRNA-seq allows us to quantify changes in the tRNA pool as part of this mechanism. We've used it extensively to validate this new model for protein translation.

Rimozione della metilazione post-trascrizionale negli RNA mediante AlkB demetilasi e successiva idrolisi ibrida RNA-cDNA nella preparazione del sequenziamento dell'RNA

Per iniziare, preparare 10 millilitri di tampone di reazione 2X AlkB e sterilizzare attraverso un filtro per siringa da 0,2 micron. In una provetta sterile per PCR, aggiungere 20 microlitri di RNA legati al linker 1, 50 microlitri del tampone di reazione 2X AlkB, due microlitri di AlkB demetilasi, un microlitro di inibitore degli RNA e 27 microlitri di RNA di acqua libera per preparare la reazione di digestione di AlkB. Incubare la miscela di digestione AlkB a temperatura ambiente per due ore per rimuovere la metilazione post-trascrizionale dagli RNA.Per la separazione in fase pulita, aggiungere 50 microlitri di acqua priva di RNA nella reazione AlkB. Quindi, aggiungi 100 microlitri di miscela di fenolo, cloroformio e alcol isoamilico. Agitare il tubo per 10 secondi.Centrifugare la miscela di AlkB a 16.000 g per 10 minuti. Trasferire circa 140 microlitri di RNA contenenti lo strato acquoso superiore in una provetta sterile da 1,5 millilitri. Per rimuovere il fenolo residuo, aggiungere 100 microlitri di cloroformio agli RNA estratti e agitare il tubo.Centrifugare la miscela a 16.000 G per 10 minuti e trasferire circa 120 microlitri dello strato acquoso superiore in una provetta sterile da 1,5 millilitri. Dopo la reazione di trascrizione inversa, aggiungere un microlitro di idrossido di sodio a cinque molari nell'ibrido RNA cDNA. Incubare a 93 gradi Celsius per tre minuti per idrolizzare il filamento di RNA dell'ibrido di RNA cDNA.Quindi, aggiungere 0,77 microlitri di acido cloridrico a cinque molari per neutralizzare la reazione. Preparare un gel di agarosio al 3% in tampone TAE. Mescolare un microlitro di colorante di carico 6X in cinque microlitri di prodotto PCR e caricare il gel con la miscela.Caricare cinque microlitri di 50 o 100 coppie di basi DNA nel pozzetto prima del primo campione e nel pozzetto dopo l'ultimo campione. Eseguire l'elettroforesi su gel a 120 volt e 400 milliampere per 75 minuti per individuare i prodotti PCR. Dopo l'elettroforesi, posizionare il gel in una scatola e riempirla con acqua deionizzata fino a quando il gel non è completamente immerso.Aggiungere 10 microlitri di bromuro di etidio nell'acqua. Avvolgere la scatola con un foglio di alluminio e colorare per 30 minuti su uno shaker. Gettare l'acqua contenente bromuro di etidio in una bottiglia di scarto posta in una cappa aspirante.Sciacquare una volta il gel con acqua deionizzata e gettare l'acqua in una bottiglia di rifiuti. Dopo aver lavato il gel con acqua deionizzata per 10 minuti, utilizzare un gel imager per visualizzare le bande e acquisire un'immagine ad alta risoluzione del gel.

post-transcriptional-methylation-removal-rnas-using-alkb-demethylase

Research

JoVE Journal

Genetics

Post-Transcriptional Methylation Removal in RNAs Using AlkB Demethylase and Subsequent RNA-cDNA Hybrid Hydrolysis in RNA Sequencing Preparation

AQRNA-seq for Quantifying Small RNAs

AQRNA-seq provides a direct linear relationship between sequencing read counts and small RNA copy numbers in a biological sample, thus enabling accurate quantification of the pool of small RNAs. The AQRNA-seq library preparation procedure described here involves the use of custom-designed sequencing linkers and a step for reducing methylation RNA modifications that block reverse transcription processivity, which results in an increased yield of full-length cDNAs. In addition, a detailed implementation of the accompanying bioinformatics pipeline is presented. This demonstration of AQRNA-seq was conducted through a quantitative analysis of the 45 tRNAs in Mycobacterium bovis BCG harvested on 5 selected days across a 20-day time course of nutrient deprivation and 6 days of resuscitation. Ongoing efforts to improve the efficiency and rigor of AQRNA-seq will also be discussed here. This includes exploring methods to obviate gel purification for mitigating primer dimer issues after PCR amplification and to increase the proportion of full-length reads to enable more accurate read mapping. Future enhancements to AQRNA-seq will be focused on facilitating automation and high-throughput implementation of this technology for quantifying all small RNA species in cell and tissue samples from diverse organisms.

Absolute quantification RNA sequencing (AQRNA-seq) is a technology developed to quantify the landscape of all small RNAs in biological mixtures. Here, both the library preparation and data processing steps of AQRNA-seq are demonstrated, quantifying changes in the transfer RNA (tRNA) pool in Mycobacterium bovis BCG during starvation-induced dormancy.

AQRNA-seq provides a direct linear relationship between sequencing read counts and small RNA copy numbers in a biological sample, thus enabling accurate ...

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Genetica

To begin, prepare 10 milliliters of 2X AlkB reaction buffer and sterilize through a 0.2 micron syringe filter. In a sterile PCR tube, add 20 microliters of the linker 1-ligated RNAs, 50 microliters of the 2X AlkB reaction buffer, two microliters of the AlkB demethylase, one microliter of RNAs inhibitor, and 27 microliters of RNAs free water to prepare AlkB digestion reaction. Incubate the AlkB digestion mixture at room temperature for two hours to remove post-transcriptional methylation from the RNAs.For clean phase separation, add 50 microliters of RNAs-free water into the AlkB reaction. Then, add 100 microliters of phenol, chloroform, and isoamyl alcohol mixture. Shake the tube for 10 seconds.Centrifuge the AlkB mixture at 16, 000G for 10 minutes. Transfer approximately 140 microliters of the top aqueous layer-containing RNAs into a sterile 1.5 milliliter tube. To remove residual phenol, add 100 microliters of chloroform to the extracted RNAs and shake the tube.Centrifuge the mixture at 16, 000G for 10 minutes and transfer approximately 120 microliters of the top aqueous layer into a sterile 1.5 milliliter tube. After reverse transcription reaction, add one microliter of five molar sodium hydroxide into the RNA cDNA hybrid. Incubate at 93 degrees Celsius for three minutes to hydrolyze the RNA strand of the RNA cDNA hybrid.Then, add 0.77 microliters of five molar hydrochloric acid to neutralize the reaction. Prepare a 3%agarose gel in TAE buffer. Mix one microliter of 6X loading dye into five microliters of PCR product, and load the gel with the mixture.Load five microliters of 50 or 100 base pair DNA ladders into the well before the first sample and the well after the last sample. Run gel electrophoresis at 120 volts and 400 milliamperes for 75 minutes to locate the PCR products. After electrophoresis, place the gel in a box and fill it with deionized water until the gel is completely immersed.Add 10 microliters of ethidium bromide into the water. Wrap the box with foil, and stain for 30 minutes on a shaker. Discard the ethidium bromide-containing water into a waste bottle placed in a fume hood.Rinse the gel with deionized water once and discard the water into a waste bottle. After washing the gel with deionized water for 10 minutes, use a gel imager to visualize the bands and acquire a high resolution image of the gel.