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The importin-ß P446L dominant-negative mutant protein loses RanGTP binding ability and blocks the formation of intact nuclear envelope

Gyula Timinszky^1,*, László Tirián^1,*, Ferenc T. Nagy^1,4, Gábor Tóth², András Perczel³, Zsuzsanna Kiss-László¹, Imre Boros⁴, Paul R. Clarke⁵ and János Szabad^1,

¹ The University of Szeged, Faculty of Medicine, Department of Biology, Somogyi B. u. 4, H-6720 Szeged, Hungary
² The University of Szeged, Faculty of Medicine, Department of Chemistry, Szeged, Hungary
³ Department of Organic Chemistry, Eötvös Loránd University, Budapest, Hungary
⁴ Biological Research Center of the Hungarian Academy of Sciences, Szeged, Temesvári krt. 62, H-6720, Hungary
⁵ Biomedical Research Center, University of Dundee, Level 5, Ninewells Hospital and Medical School, Dundee, DD1 9SY, UK
^* These authors contributed equally to this work

View larger version (107K): [in a new window]   Fig. 1. Effects of the wild-type (A-C) and the P446L mutant importin-ß (D-F) following their injection, along with a fluorescent nuclear substrate, into wild-type cleavage embryos. Arrows show the site of injection. Import of the fluorescent nuclear substrate into the nuclei was followed in a laser-scanning microscope. The A and D, the B and E and the C and F photographs were taken at roughly identical stages of the cleavage cycles. The few nuclei shown on F appeared following diffusion of the fluorescent substrate away from the site of injection. Bar, 100 µm.

View larger version (110K): [in a new window]   Fig. 2. Effects of P446L mutant importin-ß on cleavage chromatin following its injection into wild-type cleavage embryos expressing histone-GFP. Approximately 200 picolitres P446L protein solution (1.2 µM, approximately the endogenous importin-ß concentration) was injected into the posterior end of a wild-type cleavage embryo in which histone-GFP highlighted chromatin. Chromatin organization was followed in a laser-scanning microscope. Optical sections from the anterior (A-C) and the posterior (D-F) regions of the same embryo are shown. While the anterior section was devoid of P446L, the P446L mutant protein was present at the posterior region. A and D represent interphase chromatin following P446L protein injection. B and E show segregating chromosomes. C and F show chromatin during the upcoming interphase. Note that the nuclei doubled in number and the chromosomes segregate both at the anterior (control) and posterior (`experimental') regions of the embryo. Bar, 20 µm.

View larger version (88K): [in a new window]   Fig. 3. Effect of P446L importin-ß on cleavage mitotic spindle organization. Wild-type (A-D) or P446L mutant importin-ß (E-H) solution was injected into cleavage Drosophila embryos expressing tubulin-GFP fusion protein. While mitotic spindle assembly, elongation and disassembly is not affected by the injected wild-type (A-C) and P446L (E-G) importin-ß, the tubulin-GFP protein is homogeneously distributed in the site of P446L injection indicating the failure of NE assembly (H). Tubulin-GFP is excluded from the nuclei and appear as dark holes on the optical sections (D). Bar, 10 µm.

View larger version (160K): [in a new window]   Fig. 4. Localization of the chromatin (as revealed by GFP-tagged histone; A,C) and the red-fluorescent 170 kDa TRITC-dextrane (B,D) in cleavage embryos injected with wild-type (A,B) or with P446L mutant importin-ß (C,D). Following the injection of wild-type importin-ß, the TRITC-dextrane is excluded from the nuclei that form following mitosis (B). However, following the injection of P446L, the TRITC-dextrane is not excluded from the region of the chromatin following mitosis (D), an indication of the absence of functional NE. Note that the chromatin morphology is hardly affected (C). Bar, 20 µm.

View larger version (101K): [in a new window]   Fig. 5. Cleavage embryos expressing lamin-GFP were injected at the posterior end (arrows) with wild-type (A-C) or P446L mutant importin-ß (D-F). A and D show localization of lamin-GFP during interphase following injection. The lamin-GFP molecules highlight the NE. Embryos are in metaphase in B and E, and the spindle envelopes are not affected (B,E). During the upcoming interphase, nuclear lamina re-forms in the embryos that were injected with normal importin-ß (C). No nuclear lamina assembles at the site of injection of the P446L mutant importin-ß revealing the failure of intact NE formation (F). Bar, 50 µm.

View larger version (78K): [in a new window]   Fig. 6. Nuclear import complexes form and dock on the NE of the digitonin-permeabilized HeLa cells following the addition of either wild-type (A) or P446L mutant importin-ß (C) in the presence of the fluorescent IBB-nucleoplasmin fusion protein. Upon addition of the import mixture (the fluorescent IBB-nucleoplasmin fusion protein, Ran, NTF2, RanGAP, RanBP1 and energy supply) and the wild-type importin-ß, nuclear import complexes form and enter the nuclei (B). However, when P446L mutant importin-ß is added along with the import mixture, import complexes do not form and the HeLa cell nuclei are not highlighted by fluorescent signal (D). Bar, 10 µm.

View larger version (24K): [in a new window]   Fig. 7. RanGDP removes higher amounts of importin-ß from extracts of KetelD eggs than from extracts of wild-type (WT) eggs. RanQ69L protein binds higher amounts of importin-ß protein from WT egg extract than from extract of KetelD eggs. GST protein was used as a negative control (A, left). RanQ69L protein removes high amounts of purified WT importin-ß but not purified P446L mutant protein. At the same time RanGDP removes higher amounts of purified P446L importin-ß compared with the purified WT importin-ß (A, right). More Ran is precipitated with the anti-Ketel antibody from extracts of the KetelD eggs than from extracts of WT eggs. (B, left). However, if an energy-regenerating system and 3 µM (10 times the endogenous importin-ß concentration in the extract) purified wild-type or P446L mutant importin-ß are added to WT egg extract, more Ran is precipitated from the extract supplemented with WT importin-ß (B, right). Wild-type importin-ß inhibits both exchange of the labeled GTP from Ran (C) and GTP hydrolysis (D), whereas P446L mutant importin-ß has no effect on both nucleotide exchange and GTP hydrolysis. In C, the time course of nucleotide exchange is shown on a semi-logarithmic scale and D shows the results of the reactions performed in duplicate.

View larger version (24K): [in a new window]   Fig. 8. CD spectra of model peptides representing wild-type (A) and P446L mutant importin-ß (B). The CD spectra were recorded in 100% trifluoro-ethanol (TFE, continuous lines), in a mixture of 66% TFE and 33% H2O (dashed lines), and in 33% TFE and 66% H2O (dotted lines).

View larger version (47K): [in a new window]   Fig. 9. Computer modeling of the structure of model peptides (A,C) and importin-ß (B,D) with Pro (A,B) and Leu (C,D) in the linker region between HEAT repeats 10 and 11. In computing the structure of the peptides and the proteins only three angles were changed as shown on the figure. Leu439 and Leu440 are Ile444 and Ile445 in Drosophila. Pro, Leu and Ser in the critical position appear dark blue, light blue and yellow, respectively.