AI Article Synopsis

  • LINE-1 (L1) retrotransposons create diverse ribonucleoproteins (RNPs) during their replication and the host's efforts to limit them, but their exact makeup is still not well understood.
  • The composition of L1-associated macromolecules varies according to factors like the L1 life cycle stage, whether it’s dealt with productively or suppressed, and the specific cell type involved.
  • This chapter presents techniques for identifying and analyzing the protein and RNA components of L1 macromolecules from tissues, using embryonal carcinoma cell lines (like N2102Ep) and colorectal cancer tissues as primary examples.

Article Abstract

During their proliferation and the host's concomitant attempts to suppress it, LINE-1 (L1) retrotransposons give rise to a collection of heterogeneous ribonucleoproteins (RNPs); their protein and RNA compositions remain poorly defined. The constituents of L1-associated macromolecules can differ depending on numerous factors, including, for example, position within the L1 life cycle, whether the macromolecule is productive or under suppression, and the cell type within which the proliferation is occurring. This chapter describes techniques that aid the capture and characterization of protein and RNA components of L1 macromolecules from tissues that natively express them. The protocols described have been applied to embryonal carcinoma cell lines that are popular model systems for L1 molecular biology (e.g., N2102Ep, NTERA-2, and PA-1 cells), as well as colorectal cancer tissues. N2102Ep cells are given as the use case for this chapter; the protocols should be applicable to essentially any tissue exhibiting endogenous L1 expression with minor modifications.

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Source
http://dx.doi.org/10.1007/978-1-0716-2883-6_12DOI Listing

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