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Transferrin Receptor Mrna Interactions Contributing to Iron Homeostasis

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Transferrin Receptor Mrna Interactions Contributing to Iron Homeostasis Downloaded from rnajournal.cshlp.org on October 1, 2021 - Published by Cold Spring Harbor Laboratory Press Transferrin receptor mRNA interactions contributing to iron homeostasis DHWANI N. RUPANI and GREGORY J. CONNELL Department of Pharmacology, University of Minnesota, Minneapolis, Minnesota 55455, USA ABSTRACT The transferrin receptor is the primary means of iron importation for most mammalian cells and understanding its regulatory mechanisms is relevant to hematologic, oncologic, and other disorders in which iron homeostasis is perturbed. The 3′ UTR of the transferrin receptor mRNA contains an instability element that is protected from degradation during iron depletion through interactions of iron regulatory proteins (IRPs) with five iron-responsive elements (IREs). The structural features required for degradation and the site of IRP binding required for in situ protection remain unclear. An RNA-CLIP strategy is described here that identifies the predominant site of IRP-1 interaction within a nontransformed primary cell line. This approach avoided complications associated with the use of elevated concentrations of protein and/or mRNA and detected interactions within the native environment of the mRNA. A compensatory mutagenesis strategy indicates that the instability element at minimum consists of three non-IRE stem–loops that can function additively, suggesting that they are not forming one highly interdependent structure. Although the IREs are not essential for instability, they enhance instability when IRP interactions are inhibited. These results are supportive of a mechanism for a graded response to the intracellular iron resulting from a progressive loss of IRP protection. Keywords: endonuclease; iron homeostasis; iron-responsive elements; iron regulatory proteins; transferrin receptor INTRODUCTION the CAGWGH consensus sequence, where W is A or U and H is A, C, or U (for review, see Kuhn 2015). The IRE-binding In most organisms the coordination chemistry and redox site of IRP-1 is occluded under iron-replete conditions by potential of iron in its ferrous and ferric forms are essential an iron–sulfur cluster, and the disassembly of this cluster for several key processes including DNA replication, energy under iron-deplete conditions is believed to be a major generation, and oxygen transport. Conversely, high concen- mechanism of regulating the RNA binding of IRP-1. trations of iron can generate reactive oxygen species through However, IRP-1 can also be regulated through ubiquitin- the Fenton reaction, which have been associated with an dependent degradation mediated by FBXL5, an iron-respon- increased incidence of a wide range of pathologies including sive E3 ligase (Salahudeen et al. 2009; Vashisht et al. 2009). In oncologic and neurodegenerative disorders (for review, see contrast, IRP-2 does not appear to be regulated through Silva and Faustino 2015; Bogdan et al. 2016; Gozzelino and iron–sulfur cluster assembly but is instead regulated primar- Arosio 2016). As a result, homeostatic mechanisms are ily through the FBXL5 ligase. In addition to iron, the IRE- required to ensure that sufficient but nontoxic levels of binding of both IRPs can be influenced by hypoxia, nitric iron are maintained at both the cellular and whole organism oxide, oxidative stress, and phosphorylation (for review, see levels. Anderson et al. 2012). The IRE–IRP system is essential, as The import, export, utilization, and storage of iron in indicated by the embryonic lethality of mice lacking both mammalian cells are largely regulated through the interac- IRPs (Smith et al. 2006; Galy et al. 2008). tion of iron regulatory protein-1 (IRP-1) and iron regulatory The IRE–IRP interaction can function to either modulate protein-2 (IRP-2) with mRNAs that contain an iron-respon- mRNA translation or stability, depending on the location of sive element (IRE). The function of some IREs can also be ′ the IRE. When the IRE is within the 5 UTR, IRP binding altered through a direct interaction with Fe2+ (Ma et al. 2012). The canonical IRE has a hairpin loop structure with a bulged C five base pairs from a hairpin loop containing © 2016 Rupani and Connell This article is distributed exclusively by the RNA Society for the first 12 months after the full-issue publication date (see http://rnajournal.cshlp.org/site/misc/terms.xhtml). After 12 months, it is Corresponding author: [email protected] available under a Creative Commons License (Attribution-NonCommercial Article published online ahead of print. Article and publication date are at 4.0 International), as described at http://creativecommons.org/licenses/ http://www.rnajournal.org/cgi/doi/10.1261/rna.056184.116. by-nc/4.0/. RNA 22:1–12; Published by Cold Spring Harbor Laboratory Press for the RNA Society 1 Downloaded from rnajournal.cshlp.org on October 1, 2021 - Published by Cold Spring Harbor Laboratory Press Rupani and Connell blocks translation through inhibition of A small ribosomal subunit recruitment to 1. Growth under iron α-IRP-1 the cap complex (Muckenthaler et al. deplete/replete conditions 5. Immunoprecipitation RBP 1998). The mRNAs containing a well- AAA 2. IRP-1 6. UV cross-linking RBP RNA isolation/adapter ligation IRP-1 characterized functional IRE within the AAA RBP 3. Cell lysis RBP 7. RT-PCR ′ AAA RBP 5 UTR include those encoding the fol- AAA 4. Partial RNase digest 8. Next-gen sequencing lowing: the ferritin light and heavy chains, which are the major iron-storage pro- B C -IRP-1 IgG G G G teins; ferroportin, the only identified cel- A U-3920 A U A U C G C G C G lular exporter of iron; erythroid 5- U A U G C AU A U eluted eluted sup sup pre A U G C A U aminolevulininate synthase, which cata- G U A U G C IRP-1 IRE G C G C G C lyzes the initial step of heme biosynthesis; G C G C G C IRP-2 IRE C C C and HIF2α, a major modulator of the 3910-U A U A U A AU A U A U U A-3930 U A U A hypoxic response (for review, see U A G U U A A U U A U Anderson et al. 2012). In contrast, the D Endogenous HUVEC mRNA CG C G AU A U U U U U transferrin receptor (TFRC) mRNA con- 0.05 2.5 C A G U U A U U A G C ′ u (n=6) A a G C A tains five IREs within the 3 UTR, and IRP (n=3) 3900-U a A A A u 0.04 2.0 C a C C U interactions in this region impact mRNA C g-3940 A U G c ′ U a C a U a-4052 stability. The 3 UTR that is essential and 0.03 1.5 A a c a-4006 G A c a G C a 3959-u G sufficient for iron-responsive mRNA 0.02 1.0 A a a TFRC/RPL4 C g 4005-a stability has been minimized to a 245- TFRC/POLR2A u g-3947 0.01 0.5 g u nucleotide (nt) region that contains three u (n=6) (n=3) 3887-u of the five IREs, and IRP binding to these DFO (M): 100 100 (IRE C) (IRE D) (IRE E) sites has been proposed in some manner FAC (g/ml): 15 15 TFRC mRNA (NM 003234.2) to inhibit access to an endonuclease FIGURE 1. Identifying the in situ sites of IRP-1 interaction with the TFRC mRNA. (A) The (Casey et al. 1988; Mullner and Kuhn RNA-CLIP strategy used to identify sites of IRP-1 interaction. The immunoprecipitation step 1988). Despite this mechanism having enriched for IRP-1 and associated crosslinked RNAs relative to unrelated RNA binding proteins being proposed over 25 years ago, the (RBP). (B) The anti-IRP-1 polyclonal antibody exploited for the RNA-CLIP immunoprecipitates – – means through which IRP binding stabil- IRP-1 IRE complexes but not IRP-2 IRE complexes. One picomol of each recombinant IRP was UV crosslinked to a radiolabeled 43-nt IRE transcript for direct loading on the gel (pre) or incu- izes the TFRC mRNA, the nature of the bation with either anti-IRP-1 polyclonal or control rabbit IgG antibody that had been bound to endonuclease recognition element, and magnetic beads. The nonbound complexes in the supernatant (sup) and the complexes eluted the identity of the endonuclease remain from the beads, by heating in gel-loading buffer after two washes in lysis buffer, are indicated. unclear. Here, we identify the major site Gels are representative of three sets of reactions. (C) IRP-1 interacting sites identified by the RNA-CLIP. Upper case letters represent the most abundant CLIP sequences and lower case the of the IRP-1 interaction occurring with longest 3′ and 5′ extensions present within the nine libraries. (D) The TFRC mRNA level in the TFRC mRNA in situ, and show that HUVECs is iron-responsive. Cells were treated with either DFO or FAC for 14 h prior to the iso- the instability element consists of three lation of total RNA. Both RPL4 and POLR2A were used as qRT-PCR reference amplicons. 5-bp hairpin loops that can function additively. The study expands upon an earlier model for iron-responsive regulation and provides a the coimmunoprecipitation (step 5 of Fig. 1A) was raised mechanism for a graded response to a loss of IRP protection. against full-length human IRP-1. Although the anti-IRP-1 polyclonal quantitatively binds crosslinked IRP-1–IRE com- plexes, the avidity is not sufficient to recover any detectable RESULTS IRP-2–IRE complexes from the immunoprecipitation (Fig. 1B). As a result, the RNA-CLIP strategy should only identify RNA-CLIP identifies sites of in situ IRP-1 interaction IRP-1 interactions.
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