ED’AMICO and others Kif3a and thyroid function 50:3 375–387 Research Thyroid-specific inactivation of KIF3A alters the TSH signaling pathway and leads to hypothyroidism Eva D’Amico1, Ste´phanie Gayral1, Claude Massart2, Jacqueline Van Sande2, Jeremy F Reiter3, Jacques E Dumont2, Bernard Robaye1 and Ste´phane Schurmans1,4,5,6 1Institut de Recherche Interdisciplinaire en Biologie Humaine et Mole´ culaire (IRIBHM), Institut de Biologie et de Me´ decine Mole´ culaires (IBMM), Universite´ Libre de Bruxelles (ULB), Rue des Professeurs Jeener et Brachet 12, 6041 Gosselies, Belgium 2IRIBHM, Universite´ Libre de Bruxelles (ULB), Campus Erasme, Route de Lennik 808, 1070 Brussels, Belgium 3Department of Biochemistry and Biophysics, University of California, Smith Cardiovascular Research Building, Mission Bay Boulevard South 555, San Francisco, California 94158-9001, USA 4Laboratoire de Ge´ ne´ tique Fonctionnelle, GIGA-Research Centre, Universite´ de Lie` ge (ULg), Rue de l’Hoˆ pital 1, Correspondence 4000 Lie` ge, Belgium should be addressed 5Welbio, Universite´ de Lie` ge, Lie` ge, Belgium to S Schurmans 6Secteur de Biochimie Me´ tabolique, De´ partement des Sciences Fonctionnelles, Universite´ de Lie` ge, Boulevard de Email Colonster 20, 4000 Lie` ge, Belgium [email protected] Abstract Kinesins, including the kinesin 2/KIF3 molecular motor, play an important role in intracellular Key Words traffic and can deliver vesicles to distal axon terminals, to cilia, to nonpolarized cell surfaces or to " thyroid epithelial cell basolateral membranes, thus taking part in the establishment of cellular polarity. " hypothyroidism We report here the consequences of kinesin 2 motor inactivation in the thyroid of 3-week-old " genetically-modified mouse C C Kif3aD/flox Pax8Cre/ mutant mice. Our results indicate first that 3-week-old Pax8Cre/ mice used " Kif3a Journal of Molecular Endocrinology in these experiments present minor thyroid functional defects resulting in a slight increase in " molecular motor circulating bioactive TSH and intracellular cAMP levels, sufficient to maintain blood thyroxine " kinesin 2 levels in the normal range. Second, Kif3a inactivation in thyrocytes markedly amplified the phenotype observed in Pax8Cre/C mice, resulting in altered TSH signaling upstream of the second messenger cAMP and mild hypothyroidism. Finally, our results in mouse embryonic fibroblasts indicate that Kif3a inactivation in the absence of any Pax8 gene alteration leads to altered G protein-coupled receptor plasma membrane expression, as shown for the b2 adrenergic receptor, and we suggest that a similar mechanism may explain the altered TSH D/flox Cre/C Journal of Molecular signaling and mild hypothyroidism detected in Kif3a Pax8 mutant mice. Endocrinology (2013) 50, 375–387 Introduction Little is known about molecular motors responsible hormones, the TSH receptor and the sodium/iodide for intracellular traffic in thyroid follicle cells. However, symporter (NIS) must reach the basolateral surface, like in other polarized cells, thyroid proteins must while thyroperoxidase and the dual oxidases must be specifically reach the apical or basolateral membrane transported to the thyrocyte apical membrane, and to be functional. In order to assure the synthesis of thyroglobulin (TG) exported through the apical mem- tri-iodothyronine (T3)andthyroxine(T4)thyroid brane in the colloid. http://jme.endocrinology-journals.org Ñ 2013 Society for Endocrinology Published by Bioscientifica Ltd. DOI: 10.1530/JME-12-0219 Printed in Great Britain Downloaded from Bioscientifica.com at 09/28/2021 09:28:13PM via free access Research ED’AMICO and others Kif3a and thyroid function 50:3 376 Kinesins play an important role in intracellular traffic. Ethical Committee of the Medical and the Sciences School The superfamily of kinesins is constituted of motor of the Universite´ Libre de Bruxelles. proteins that use energy liberated from ATP hydrolysis to transport vesicles along microtubules. These proteins are Genotyping and analysis of Cre/lox recombination composed of a motor domain containing an ATP-binding specificity site and a microtubule-binding site, a domain that binds vesicles, and an oligomerization domain (Scholey 1996). PCR was performed on tail DNA with oligonucleo- Most of these motor proteins, including kinesin 2, mediate tide primers 1 (50-AGGGCAGACGGAAGGGTGG-30), vesicle transport over long distances to the plus end of 2(50-TCTGTGAGTTTGTGACCAGCC-30), and 3 (50-TGGC microtubules. This transport pathway is highly conserved AGGTCAATGGACGCAG-30). Using these three primers in through evolution. In view of microtubule organization, the same PCR, amplicons of 200, 360, and 490 bp were kinesins can deliver vesicles to distal axon terminals, obtained, corresponding to the delta, wild-type, and to cilia or flagella, to nonpolarized cell surfaces or to floxed Kif3a allele respectively. epithelial cell basolateral membranes, taking part in the establishment of cellular polarity (Hirokawa 2000). Cell culture Kinesin 2 motor (or kinesin family member 3 (KIF3)) is C C K K Large T antigen-immortalized Kif3a / and Kif3a / composed of a heterotrimeric complex KIF3A–KIF3B– KAP3. KIF3A/KIFB are the motor proteins and KAP3 mouse embryonic fibroblasts (MEFs) were maintained in m regulates the binding between the cargo and the KIF3 DMEM supplemented with 100 U/ml penicillin, 100 g/ml heterodimer (Hirokawa 2000). This molecular motor is streptomycin, 15% fetal bovine serum, 1.1 mM sodium L m expressed in all tissues, including the thyroid. KIF3A or pyruvate, 3.97 mM -glutamine, 100 M nonessential m KIF3B inactivation in mice leads to abolition of molecular amino acids and 300 g/ml G418 (Sigma–Aldrich). Cells motor function and to an early embryonic lethality. were kept in a humidified incubator at 37 8C and 5% CO2. These knockout embryos exhibit loss of cilia ordinarily The medium was changed every 3 days. present on cells of the embryonic node, leading to a randomized establishment of left–right asymmetry and Western blotting numerous structural abnormalities (Nonaka et al. 1998, Thyroid and MEF proteins were extracted using RIPA buffer Marszalek et al. 1999). (Tris–HCl50mM,pH7.4,EDTA1mM,NaCl150mM,Triton In this study, we have explored the role of the kinesin 2 X-100 1%, Sodium deoxycholate 1%, SDS 0.1%). Thyroid Journal of Molecular Endocrinology molecular motor in mouse thyroid development, structure (25 mg) and MEF (60 mg) protein extracts were separated on a and function 3 weeks after birth. We used mice carrying a 10% SDS–PAGE and transferred onto PVDF membrane Kif3a floxed gene as well as knock-in mice expressing the (Amersham Biosciences) using a Mini Trans-Blot Transfer Cre recombinase under the control of the endogenous Cell system (Bio-Rad). Membrane was preincubated for 1 h et al et al Pax8 promoter (Marszalek . 1999, Bouchard . with 5% milk and 0.1% Tween in PBS, followed by overnight Cre/C 2004). Indeed, in these Pax8 mice, the expression of incubation at 4 8C with a Kif3a antibody (Sigma–Aldrich) the recombinase mimics the expression of the paired diluted 1:2000, or with a b-actin antibody (Sigma–Aldrich) domain transcription factor Pax8, including thyroid diluted 1:5000, or with a b2 adrenergic receptor (ADRB2) follicle cells, kidney, inner ear, and the mid–hindbrain antibody (Abcam, Cambridge, UK) diluted 1:1000 in the boundary region, all of them from the embryonic stage same buffer. The membrane was washed in PBS and then E8.5 (Plachov et al. 1990, Bouchard et al. 2002). incubated for 1 h at room temperature with peroxidase- conjugated protein A (Sigma–Aldrich) diluted 1:10 000. Proteins were visualized with Western Lightning plus-ECL Materials and methods (Perkin-Elmer) and exposed to X-ray film. Protein concen- Mice tration was determined with Bio-Rad protein assay reagents using BSA as standard. Kif3aD/flox mice, obtained from LS Goldstein (University of C California, San Diego, USA) and Pax8Cre/ mice, obtained Serum hormone assays from M Busslinger (Research Institute of Molecular Path- ology, Vienna, Austria) were on a mixed Sv129!C56BL/6 Enzyme immunoassays for mouse T3 and T4 were genetic background. All procedures were approved by the performed using Mouse/Rat T3 ELISA kit from Calbiotech http://jme.endocrinology-journals.org Ñ 2013 Society for Endocrinology Published by Bioscientifica Ltd. DOI: 10.1530/JME-12-0219 Printed in Great Britain Downloaded from Bioscientifica.com at 09/28/2021 09:28:13PM via free access Research ED’AMICO and others Kif3a and thyroid function 50:3 377 (Spring Valley, SK, Canada) and T4 ELISA kit from Immunohistochemistry DiaSource (Louvain-la-Neuve, Belgium) respectively. For TG analysis, sections were deparaffinized and treated TSH was measured in a bioassay using a line of with 0.3% hydrogen peroxide in methanol for 30 min. Chinese hamster ovary cells stably transfected with the They were incubated with blocking solution (10% goat human TSH receptor cDNA, as previously described (Perret serum in PBS) for 1 h and then with a human TG antibody et al. 1990, Moeller et al. 2003). Briefly, 50 000 cells (Dako, Heverlee, Belgium) diluted 1:2500 overnight at were seeded in individual test tubes and incubated for room temperature. 24 h in 100 ml Ham’s F-12 nutrient mixture supplemented For iodinated TG analysis, quenching of endogenous with 10% FCS, 100 IU/ml penicillin, 100 mg/ml strepto- peroxidases was performed, and then antigen retrieval was mycin, 1 mM sodium pyruvate and 2.5 mg/ml Fungizone. done by boiling the slides immersed in citrate buffer at pH 6. Cells were washed with 500 ml Krebs-Ringer HEPES They were incubated with blocking solution (10% BSA/2% buffer (pH 7.4), supplemented with 8 mM glucose and sheep serum in PBS) for 1 h and then with an antibody 0.5 g/l BSA and then preincubated for 30 min in 200 mlof directed against iodinated TG (a kind gift from Prof. thesamemedium.Themediumwasremovedand C Ris-Stalpers, Laboratory of Pediatric Endocrinology, 200 mloffreshbuffercontaining20mlofserumfor Amsterdam, The Netherlands) diluted 1:2000 overnight at 4 8C.
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