Neuroscience

The ciliary kinesin KIF7 controls the development of the cerebral cortex by acting differentially on SHH-signaling in dorsal and ventral forebrain

María Pedraza
Valentina Grampa
Sophie Scotto-Lomassese
Julien Puech
Aude Muzerelle
Azka Mohammad
Sophie Lebon
Nicolas Renier
Christine Métin
Justine Masson author has email address

INSERM, UMR-S1270, Institut du Fer à Moulin, Sorbonne Université, Paris, France
Université Paris Cité, NeuroDiderot, Inserm UMR1141, Paris, France
Institut du Cerveau et de la Moelle Épinière, Laboratoire de Plasticité Structurale, Sorbonne Université, INSERM U1127, CNRS UMR7225, Paris, France

https://doi.org/10.7554/eLife.100328.2

Open access
Copyright information

Figures and data

Clinical diagnosis of patients carrying mutation in the KIF7 gene on both alleles from the literature.
The ablated or mutated domains were identified. Clinical features associated with cortical dysfunction are listed. Among cerebral defects, those observed in the cortex are enlighted. DD, developmental delay; ID, intellectual deficit; CC, corpus callosum; MTS, molar tooth sign.

Kif7 deletion alters cortical development on latero-medial and rostro-caudal axes.
(A) Kif7 -/- embryos are microphtalmic (black arrow) and exhibit skin laxity (white arrow). (B) External examination of the brain reveals the lack of olfactory bulbs (white arrows, left panel) and the thinning of the dorsal telencephalon (black arrow, right panel). (C) DAPI staining of rostro-caudal series of coronal sections at E12.5 (C1), E14.5 (C2) and E16.5 (C3) illustrates the anatomical defects of Kif7 -/- embryonic brains quantified at E14.5 in C4. The ventricles of Kif7 -/- embryos are strongly enlarged (upper left graph; WT, n=4-6, Kif7 -/-, n=5-6 depending on the rostro-caudal level), their cortical thickness strongly decreased (upper right graph; (WT, n=3; Kif7 -/-, n= 4), resulting in minimal brain width (lower left graph; WT, n=5-6; n=5-6 for Kif7 -/- depending on the rostro-caudal level) and height (lower right graph; WT, n=5-6; Kif7 -/-, n=4-6 depending on the rostro-caudal level) changes. Statistical significance was tested by Two-way ANOVA or mixed model (GraphPad 8.1.0). For ventricle surface and cortex thickness, mix model reveals a genotype effect (p<0.0001). For brain width and height, no genotype effect was observed, but a significant effect of the rostro-caudal level on brain width (P=0.0441) and height (P=0.0092). (D) The pallium-subpallium boundary identified by the limit of expression of ventral (GSH2, D1, D2) and dorsal (TBR2, D3, D4) telencephalic markers is less precisely defined and slightly shifted to the ventricular angle in E13-E14 Kif7 -/- embryos compared to wild type embryos (epifluorescent low magnification, D1, D3; confocal high magnification images, D2, D4). Graphs in C4 represent the means and S.E.M. Cx, cortex; Hip, hippocampus; LGE, lateral ganglionic eminence; MGE, median ganglionic eminence; CGE, caudal ganglionic eminence; Th, thalamus.. Scale bars, 500 µm (C,D1,D3), 150 µm (D2,D4).

Western blot analysis on the cortex and MGE of wild type (WT) and Kif7 -/- embryos at E14.5.
(A) The clived form of GLI3 (GLI3-R at 83 KDa) and the full length GLI3 (GLI3-FL at 190 KDa) are more abundant in the cortex compared to the MGE (see actin band intensity for protein loading). (B) The ratio Gli3-R/Gli3-FL is lower in the MGE than in the cortex of WT animals and is significantly decreased only in the cortex of Kif7 -/- brains compared to control. Two way ANOVA reveals significant interaction between brain structure and genotype (WT, n=4; Kif7 -/-, n=4; P=0.002) and multiple comparisons show a statistical difference between genotype only in the cortex (****, P<0.0001)]. Graph represents the means and S.E.M.

Histological alterations in the developing cortex of Kif7 -/- embryos.
(A-C) Immunostaining of cortical post-mitotic layers in E14.5 (A), E16.5 (B) and E18.5 (C) in median coronal sections representative of 5 WT and Kif7 -/- embryos imaged on epifluorescence (A1,B,C) or confocal (A2) microscopes. At E14.5 (A1,A2), the TBR1(+) staining (red) of the cortical plate is more clustered in Kif7 -/- than in WT embryos, and the MAP2(+) staining (green) of the subplate is absent in the dorsal cortex of E14.5 Kif7 -/- embryos (white arrow, right column). The post-mitotic layers remain thinner in Kif7 -/- embryos at later embryonic stages as illustrated by TBR1 staining at E16.5 (B) and CTIP1 staining at E18.5 (C) that specifically labels the deeper cortical layers (V-VI). Moreover, the hippocampus is underdeveloped in the mutant (white arrow) (C). (D-F) Immunostaining of TBR2(+) proliferative layer. At E14.5 (D1,D2), the TBR2(+) layer (green) of secondary progenitors appears disorganized in the lateral cortex of the Kif7 -/- embryos (white arrowhead in D1) and reaches the brain surface in the dorsal cortex of Kif7 -/- embryo where it intermingles with post-mitotic TBR1(+) cells (D2, red) (white arrows). In E12.5 Kif7 -/- embryo (E), the TBR2(+) layer is thin and clustered however its localization in the thickness of the cortex is normal. At E16.5 stage (F), the TBR2(+) layer is normally positionned in the deeper layer of the cortex in both WT and Kif7 -/- embryos. Hip, hippocampus; V, ventricle; VZ, ventricular zone; SVZ, subventricular zone; IZ, intermediate zone; CP, cortical plate; MZ, marginal zone. Scale bars: 250 µm (A1,B,F), 100 µm (A2), 200 µm (D,E); 500 µm (C).

Kif7 deletion disrupts of the connectivity between the cortex and the thalamus.
(A) Panels illustrate the corticofugal projections labeled by DiI crystal (red dots) positioned in the dorsal (A1) and lateral (A2,A3) cortex of E14.5 WT (left) and Kif7 -/- (right) embryos on vibratome sections performed 30 days after DiI placement and imaged on a macroscope. In Kif7 -/- embryos, less axons project from the dorsal (A1) and lateral (A2) cortex to the subpallium than in WT (compare enlarged views of the projections below A1 and A2). Cortical injections in Kif7 -/- embryos do not label thalamic axons (compare left and right panels in A3) but label a ventral projection (A3, white arrow). (B) Rostro-caudal series of coronal sections (B1-B5) immunostained with anti-Netrin G1a (NG1a) antibodies compare the trajectory of thalamo-cortical axons (TCA) in a E14.5 WT (left) and in a Kif7 -/- (right) embryo imaged on a macroscope. TCA reach the pallium-subpallium boundary of the WT embryo whereas they are lost in the ventral forebrain of the mutant (B4, white arrow). (C) Representative three-dimensional reconstructions (C1, lateral; C2, horizontal; C3, coronal views) of WT and Kif7 -/- E14.5 brains immunostained as a whole with NG1a (red) and TBR1 (green) antibodies that label respectively the TCA and cortical plate cells before transparization and imaging with a light sheet microscope (see Supplementary movies S1 and S2). While all labeled TCA extend in the internal capsule (IC) and a significant proportion of them enter the cerebral cortex in the WT brain, TCA in the Kif7 -/- brain split in two bundles in the basal telencephalon. A bundle stops shortly after entering the IC (white arrowheads) whereas the second bundle extends ventrally (white arrows). (D) At E16.5, TCA are immunostained with NG1a in WT (left) and Kif7 -/- (right) embryos in whole brain with TBR1 antibodies before transparization and imaging (D1) and on coronal section with TBR2 (D2). The TCA extend in the cortex in Kif7 -/- brain, however, fiber density is reduced in the median and caudal brain compared to WT (D1, white arrowhead). TCA invade the post mitotic layers in the cortex (above TBR2 layer) to a lower extend in Kif7 -/- brain (D2). In the Kif7 -/- brain, thick bundles of NG1a(+) fibers project ventrally from the caudal telencephalon, a projection never observed in control brains (D1, white arrow). (E) At E18.5, rostro-caudal series of coronal sections (E1-E4) immunostained with NG1a antibodies compare the trajectory of TCA in WT (left) and Kif7 -/- (right) embryos imaged on a macroscope. TCA reach the dorsal cortex in both WT and Kif7 -/- embryos. However, the TCA projection in Kif7 -/- (arrowheads) become thinner in median sections (E2) and almost disappers in caudal sections (E3,E4). Fiber trajectories in the lateral striatum are abnormal (E2,E3, arrows). (F) Panels illustrate the cortical projections immunolabeled by Smi32 antibodies in E18.5 WT and Kif7 -/- brain. In Kif7 -/- brain, the number of fibers connecting the cortex with other brain structures is strongly reduced (arrow). Cx, cortex; dTh, dorsal thalamus; Hip, hippocampus; Hy, hypothalamus; St, striatum; IC, internal capsule; LGE, lateral ganglionic eminence; MGE, median ganglionic eminence; PSB, pallium-subpallium boundary; .. Scale bars: 250 µm (A,B,C,D), 500 µm (E,F).

Abnormal cortical distribution of cIN and Cxcl12 transcript expression in E14.5 in Kif7 -/- brains.
(A) The cortical distribution of cIN is visualized in WT and Kif7 -/- mouse embryos crossed with the Nkx2.1-Cre/R26R-tdTomato strain in which MGE-derived cIN express the fluorescent marker tdTomato. Panels in A1 compare the distribution of tdTomato (+) cIN in WT and Kif7 -/- cortical sections prepared at the same rostro-caudal level and in which SVZ is immunostained with TBR2 antibodies (green). Pictures show that the deep migratory stream of cIN terminates in Kif7 -/- brains in the cortical region where the TBR2(+) layer reaches the cortical surface. Quantitative analysis of the mean length of the deep and superficial migratory streams measured from the entry in the pallium to the last detected cIN in the cortex is illustrated in graph A2. Statistical significance is assessed using Two way ANOVA [layers (WT, n=4; Kif7 -/-, n=3; ***, P=0.001) and genotype (*, P=0.0157)]. (B) Representative pictures (B1) of the deep and superficial tangential migratory streams of cIN in the lateral cortex of WT and Kif7 -/- embryos. Pictures illustrate the decreased thickness of the superficial stream, and the reduced distance between the deep-superficial streams in Kif7 -/-embryos. Graph in B2 (WT, n=4; Kif7 -/-, n=4) compares the distribution of the fluorescence intensity along a ventricle/MZ axis (see grey rectangles in B1) using the plot profile function of FIJI. Curves show no change in the distance between the ventricular wall and the deep cIN, but a significant reduction of the distance between the two streams in the Kif7 -/- cortical sections as quantified on the graph B3 [WT, n=4; Kif7 -/-, n=4; Two way ANOVA reveals a significant interaction between genotype and layer (P=0.0233) and multiple comparisons, a statistical difference between genotype only for the distance between de cIN streams (**, P=0.0051)]. (C) Panels compare the distribution of Cxcl12 mRNA in WT (left panel) and Kif7 -/- (right panel) forebrain coronal sections at E14.5. The WT section shows Cxcl12 transcript enrichment in a deep cortical layer already identified as the SVZ. In the Kif7 -/- cortical section, the expression of Cxcl12 transcripts is reduced to the lateral part of the SVZ. (D) Z-projections of 30 frames acquired during 12h in the dorsal cortex of living organoptypic forebrain slices representative of E14.5 WT and Kif7 -/- embryos with tdTomato expressing cIN. Kif7 -/- cIN were able to migrate dorsally but followed preferentially radially oriented trajectories Scale bars: 200 µm.

Dynamic behavior of migrating cIN in co culture and organotypic cortical slices.
(A) To prepare co-cultures, MGE explants were dissected out of telencephalic vesicles at E14.5 from WT or Kif7 -/- Nkx2.1-Cre;Rosa26-tdTomato embryos and placed on a substrate of WT E14.5 dissociated cortical cells (A1). After 24h in culture, MGE cells migrated centrifugally away from MGE explants on the substrate of cortical cells and were recorded for 7 hours.WT (n=160) and Kif7 -/- (n=126) MGE cells were tracked manually using the MTrackJ plugin allowing to analyze migratory parameters (A2). Box and whisker plots indicate the speed (A3), the time without nuclear movement (A4), the frequency (A5) and speed of nuclear movements (A6). Statistical significance is assessed by Mann Whitney or Unpaired tests. ***, P<0.001 (A4); *, P=0.0308 (A3), P=0.0123 (A5). Directionality persistence was calculated as the ratio of the cell displacement (distance between the first and last positions of the cell) on the cell trajectory (A7, scheme on the right). Graph represented the mean directionality ratios at each time point over the first 5 hours of recording for the recorded cells (A7). Statistical significance is assessed using Two way ANOVA and reveals a significant effect of time and genotype (****, P<0.0001)]. Scale bar: 50 µm (A2). (B) tdTomato(+) cIN migrating in living cortical slices from Nkx2.1-Cre;Rosa26-tdTomato embryos were tracked manually using the MTrackJ plugin and their trajectories color-coded as shown in legend (B2) to characterize their preferred direction (tangential, oblique, radial, immobile) and cortical layer localization (VZ-SVZ, IZ, CP).The picture in B1 illustrates the z-projection of trajectories reconstructed in a control slice, superimposed to the last picture of the movie. Cortical interneurons migrating tangentially in the superficial migratory stream (MZ) could not be tracked because of high density. Graphs in B2 compare the percentage of each kind of trajectory recorded in the lateral cortex of control slices (control, see also Suppl. Movie S3), Kif7 -/- slices (Kif7 -/-, see also Suppl. Movie S4), control slices treated acutely with either murine SHH (SHH, see also Suppl. Movie S5) or cyclopamine (Cyclo, see also Suppl. Movie S6). Significance of the differences between the four distributions were assessed by a Chi-square test, X² (24, n=1224), P=0.0004998, ***). All experimental conditions differed from the control (Fisher test, P =0.0004998, ***). Slices from three WT animals in control condition or treated with drugs and from three Kif7 -/- animals were analyzed; the number of analyzed cells is indicated above bars. Schemes in B3 summarize the main results observed in each experimental condition. Trajectories are represented with the same color code as in B1, and line thickness is proportional to the percentage of cells exhibiting each type of trajectory. Immobile cells are figured by a coil. Box and whisker plots indicate the mean speed (B4), the frequency of period without nuclear movment (number/h) (B5) and the mean duration of period without nuclear movement (hour) (B6) for cIN migrating tangentially in the deep stream (red box and whisker plots, left) or to the cortical plate (green box and whisker plots, right). Statistical significance assessed by Krustkal-Wallis tests in each cluster. ****, P<0.0001; ***, B5 left P=0.0005; **, B4 right P=0.0088, B5 right, P=0.0037, B6 left P=0.0034; *, B4 left P=0.0233, B5 right P=0.0470, B6 left P=0.0134, B6 right P=0.0394. Number of analyzed cells is indicated on plots. VZ, ventricular zone; SVZ, subventricular zone; IZ, intermediate zone; CP, cortical plate; MZ, marginal zone. Scale bar: 300 µm.

Expression of Shh transcripts (A-C) and distribution of SHH protein (D) in the E13.5-E14.5 forebrain.
(A,B) Distribution in median (A) and caudal (B) coronal sections of Shh mRNA detected by in situ hybridization with an antisens Shh probe at E13.5 (A1,B1) and by RNAscope at E14.5 (A2-3,B2). Shh transcripts are strongly expressed in the medial ventral forebrain (SVZ and mantle zone of the MGE and septum, A1, A2), in the mantle zone of the CGE (B1,B2), in the zona limitans intrathalamica (ZLI in B1) and in the ventral midline of the 3^rd ventricle (V3 in B1). RNAscope further confirmed the strong expression of Shh mRNA (A3, green) in MGE and septum regions that strongly express Lhx-6 mRNA (A2, red). Confocal observations in the SVZ and mantle zone of the MGE showed that Shh mRNA (green) is co-expressed with the Lhx6 mRNA (red) in a significant number of cIN (yellow cells in A4). (C) Confocal analyses at higher magnification of the double detection by RNAscope of Shh and Lhx-6 mRNA. Cells were identified on stacked images (Δz=1 µm) using Nomarski optic. In the lateral cortex close to the PSB (C1, z projection of 10 confocal planes) and in the dorsal cortex (C2, z projection of 10 confocal planes), a very small proportion of cells expressing Lhx-6 mRNA also express Shh mRNA (white arrows in C1,C2). Counting in the deep stream (SVZ-IZ) and in the MZ is shown in graph C3 (9-17 fields in three sections). A few progenitors in the cortical VZ express Shh mRNA at very low level (arrowhead, C1). (D) SHH-Nter and TBR2 co-immunostaining of Nkx2.1-Cre/R26R- tdTomato brain coronal sections at E14.5. Representative confocal merged stacked images (Δz=0.2 µm; 48 images) in the pallium-subpallium boundary (PSB, D1), lateral cortex (D2) and dorsal (D3) cortex revealing SHH-Nter immunostaining in blood vessels and the presence of numerous bright dots all over the cortical neuropile. On the ventricular side of the PSB and of the lateral-most part of the LGE, SHH-Nter(+) brigth elements are aligned radially. In the lateral cortical neuropile, smaller bright dots align radially in the VZ, tangentially in the SVZ- IZ, and radially in the CP. Cx, cortex; LGE, MGE and CGE, lateral, medial and caudal ganglionic eminence; CP, cortical plate; Hyp, hypothalamus; PSB, pallium-subpallium boundary; Sp, septum; Th, thalamus; V3, third ventricle; VZ, ventricular zone; SVZ, subventricular zone; IZ, intermediate zone; MZ, marginal zone. Scale bars: 500 µm (A, B), 20 µm (C), 100 µm (D).

Sign up for email alerts