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Home NEWS Science News Chemistry

CityU’s CRISPR-assisted novel method detects RNA-binding proteins in living cells

Bioengineer by Bioengineer
July 1, 2020
in Chemistry
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Credit: Photo source: DOI number: 10.1038/s41592-020-0866-0

While scientists still don’t fully understand the diverse nature of RNA molecules, it is believed that the proteins binding to them, called RNA-binding proteins, are associated with many disease formation. A research led by biomedical scientists from City University of Hong Kong (CityU) has developed a novel detection method, called CARPID, to identify binding proteins of specific RNAs in the living cells. It is expected the innovation can be applied in various cell researches, from identifying biomarkers of cancer diagnosis to detecting potential drug targets for treating viral diseases.

The research was co-led by Dr Yan Jian, Dr Zhang Liang, and Dr Chan Kui-ming who are all from the Department of Biomedical Sciences (BMS) at CityU, in collaboration with scientists mainly from Northwest University in Xi’an. Their findings were published in the scientific journal Nature Methods, titled “CRISPR-assisted detection of RNA-protein interactions in living cells”.

Binding proteins determine RNA functions

The central dogma of molecular biology suggests that DNA is transcribed to RNA and RNA is translated into protein. But actually, only about 2% of RNAs code for protein. The rest 98%, named as non-coding RNAs (ncRNA) has been regarded as “dark matter” for their yet mysterious functions.

In recent years, scientists have put many efforts into unveiling their actual functions, especially the long non-coding RNAs (lncRNA, meaning ncRNA with more than 200 nucleotides in length). LncRNA has become widely accepted as important cellular components participating in the regulation of gene expression. “LncRNA is the most interesting RNA species”, described Dr Yan. It is also the reason why the team has chosen lncRNA as the research subject.

Although lncRNA will not produce protein, they will react with proteins, and the interaction will determine their functions. Therefore, the identification of the binding proteins is crucial in understanding the lncRNA functions. However, current methods demonstrate quite some limitations, for example generating false positive signals, and cannot be done in living cells.

Two steps of CARPID: navigation and biotin-labelling

To overcome the limitations of the existing method, the research team came up with a novel method that jointly leverages the existing state-of-the-art gene-editing technology CRISPR/dCasRx system for RNA targeting, and the proximity biotin-labelling technology to identify the protein-protein interactions in living cells.

The team named the novel method CARPID, short for CRISPR-Assisted RNA-Protein Interaction Detection. “CARPID can sensitively detect binding proteins of RNAs in any lengths or concentrations whereas most other methods can only be applied to very long non-coding RNAs,” said Dr Yan.

The method is composed of two parts: navigation and proximity biotin-labelling. First, the team employed the CRISPR/CasRx system to navigate so that the CARPID components, including a “labelling tool” called BASU, can be near the targeted RNA. BASU is an engineered biotin ligase, a kind of enzyme that would add biotin (a kind of vitamin with strong binding) to proteins that bind with that targeted RNA. In this way, those proteins which are near the targeted RNA would be labelled.

After the “labelling”, the team then used a biotin-binding protein called streptavidin to identify those proteins labelled by BASU. In this way, the binding proteins were revealed easily.

High specificity and applicability for lncRNAs of different lengths

To test the specificity of CARPID, the team applied it on three different lncRNAs, namely DANCR, XIST, and MALAT1. Experiment results showed that there was not much overlapping of binding proteins. This demonstrated the high specificity and applicability of the CARPID method for lncRNAs of different lengths and expression levels.

“This high level of specificity is achieved because the navigation by CRISPR is very precise. We can even obtain the information of exactly which section of the RNA that protein binding occurred,” explained Dr Yan.

Also, CARPID would not affect the physiological condition of the targeted cell, and the cell is still alive with normal gene expression landscape after the whole process. “With this new method, we can obtain dynamic results if we check the same RNA target at different times,” added Dr Zhang.

Powered by the proteomic (analysis of the protein) technique developed by Dr Zhang, the team was able to find and validate two previously uncharacterized binding proteins of a lncRNA in mammalian cells.

Enables detection of the binding proteins of viral RNA

The team believed CARPID has broad application, including the detection of the binding proteins of viral RNA. “For example, SARS-CoV-2 is an RNA virus that causes COVID-19. Once the virus infects cells, we could apply CARPID to detect what cellular proteins are recruited by this virus for the viral life cycle. If we depleted the binding proteins, we are likely to suppress the viral replication. This information may help us identify potential antiviral drug targets,” Dr Yan elaborated.

Moreover, many lncRNAs are used as diagnostic biomarkers for cancer as they become more abundant in cancer cells than normal cells. CARPID can be applied to detect the binding proteins of these lncRNAs in cancer cells which may help find tumorigenic mechanisms and potential protein targets for cancer diagnosis or treatment.

It took the team about one year to develop CARPID and most of the experiments were done in CityU. Their next step would be trying to apply it to research on stem cell and DANCR, a lncRNA that generally works as a tumour promoter.

###

Dr Yan, Dr Zhang, and Dr Chan Kui-ming (who contributed to validating CARPID) are the corresponding authors of the paper. The co-first authors of the paper are Li Jingyu and Zhu Xiaoxuan from the BMS department, together with Yi Wenkai and Dr Wang Xi, both from Northwest University in Xi’an.

The study was supported by CityU, the National Natural Science Foundation of China, the Shenzhen Science and Technology Fund Program, Hong Kong Research Grants Council, Opening Foundation of Key Laboratory of Resource Biology and Biotechnology in Western China, the Chinese Ministry of Education and the EpiHK consortium.

Media Contact
P. K. Lee
[email protected]

Related Journal Article

http://dx.doi.org/10.1038/s41592-020-0866-0

Tags: BiochemistryBioinformaticsBiologyBiotechnologycancerCell BiologyGenesGeneticsMedicine/HealthMolecular Biology
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