Date published: 2025-10-27

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MRP-L18 Inhibitors

Chemical inhibitors of MRP-L18 function by directly targeting the mitochondrial ribosome, where MRP-L18 is localized and plays a critical role in protein synthesis. Chloramphenicol achieves this inhibition by binding to the peptidyl transferase component of the mitochondrial ribosome, thus blocking the peptide bond formation that is an essential step in the synthesis of new proteins. This action directly hampers the function of MRP-L18, as it can no longer contribute to the assembly of proteins within the mitochondria. Similarly, Linezolid binds to the mitochondrial ribosome and prevents the formation of the initiation complex necessary for the commencement of protein synthesis, directly impeding the functional contribution of MRP-L18 to the ribosomal structure. Tetracycline and Doxycycline, both binding to the 30S subunit of the mitochondrial ribosome, inhibit the attachment of aminoacyl-tRNA to the ribosomal acceptor site, which is a prerequisite for protein elongation and hence, essential for the role of MRP-L18 in protein assembly. Minocycline and Tigecycline exert their inhibitory effect on MRP-L18 by a similar mechanism, where their binding to the mitochondrial ribosome obstructs the protein synthesis process, rendering MRP-L18 unable to fulfill its function in ribosomal operations. On the other side of the ribosomal subunit, Erythromycin, Azithromycin, Clarithromycin, and Telithromycin bind irreversibly to the 50S subunit, blocking the exit tunnel of the nascent peptide chain, an action that interferes with the proper functioning of MRP-L18 as part of the ribosomal machinery. Roxithromycin also targets the 50S subunit, interrupting the synthesis of mitochondrial proteins and consequently, the role of MRP-L18. Lastly, Fusidic acid impedes the action of elongation factor G in the mitochondria, a critical participant in the translocation step of protein synthesis, thereby indirectly inhibiting the functionality of MRP-L18, which is contingent upon the successful elongation and assembly of proteins within the mitochondria.

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