A novel experimental approach for the selective isolation and characterization of human RNase MRP

RNase MRP is a ribonucleoprotein complex involved in the endoribonucleolytic cleavage of different RNAs. Mutations in the RNA component of the RNP are the cause of cartilage hair hypoplasia. Patients with cartilage hair hypoplasia are characterized by skeletal dysplasia. Biochemical purification of...

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Published inRNA biology Vol. 19; no. 1; pp. 305 - 312
Main Authors Derksen, Merel, Mertens, Vicky, Visser, Eline A., Arts, Janine, Vree Egberts, Wilma, Pruijn, Ger J. M.
Format Journal Article
LanguageEnglish
Published United States Taylor & Francis 31.12.2022
Taylor & Francis Group
Subjects
Chemical Fractionation - methods
Endoribonucleases - genetics
Endoribonucleases - isolation & purification
Endoribonucleases - metabolism
Enzyme Activation
Enzyme Assays
Gene Expression
Humans
Multiprotein Complexes - isolation & purification
Multiprotein Complexes - metabolism
Mutation
Recombinant Fusion Proteins
Research Paper
ribonucleoprotein
RNA aptamer
RNase MRP
RNase P
RNA aptamer
RNase P
RNase MRP
ribonucleoprotein
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Summary:RNase MRP is a ribonucleoprotein complex involved in the endoribonucleolytic cleavage of different RNAs. Mutations in the RNA component of the RNP are the cause of cartilage hair hypoplasia. Patients with cartilage hair hypoplasia are characterized by skeletal dysplasia. Biochemical purification of RNase MRP is desired to be able to study its biochemical function, composition and activity in both healthy and disease situations. Due to the high similarity with RNase P, a method to specifically isolate the RNase MRP complex is currently lacking. By fusing a streptavidin-binding RNA aptamer, the S1m-aptamer, to the RNase MRP RNA we have been able to compare the relative expression levels of wildtype and mutant MRP RNAs. Moreover, we were able to isolate active RNase MRP complexes. We observed that mutant MRP RNAs are expressed at lower levels and have lower catalytic activity compared to the wildtype RNA. The observation that a single nucleotide substitution at position 40 in the P3 domain but not in other domains of RNase MRP RNA severely reduced the binding of the Rpp25 protein subunit confirmed that the P3 region harbours the main binding site for this protein. Altogether, this study shows that the RNA aptamer tagging approach can be used to identify RNase MRP substrates, but also to study the effect of mutations on MRP RNA expression levels and RNase MRP composition and endoribonuclease activity.
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ISSN:1547-6286
1555-8584
DOI:10.1080/15476286.2022.2027659