Mary Antypa’s research while affiliated with University College London and other places

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Publications (4)

Figure 1: Tangential migration of interneurons into the cerebral cortex. (A) Schematic diagrams depicting the streams of migrating interneurons at E13.5. Red lines indicate the laminar positions of the PPL and IZ streams. (B) Coronal section through the cortex of an E13.5 GAD67–GFP transgenic mouse showing abundant migrating cells in the PPL and IZ streams. (C and D) Intact section through the forebrain of one hemisphere of an E13.5 GAD67–GFP transgenic mouse and after excision and capture of the PPL and IZ with a laser-capture microscope. Scale bars: (A) 100 μm; (C and D) 500 μm. Cx, cerebral cortex; LGE, lateral ganglionic eminence; VZ, ventricular zone.
Table 1 . qPCR comparing expression profiles of cell surface receptor genes that are upregulated in PPL cells as compared with IZ cells
Figure 2: Numbers of genes upregulated in the PPL (grey bars) and IZ (black bars) migratory streams at E13.5. Genes were classified into the categories listed according to their molecular function.
Figure 3: Expression of receptor genes in the interneuron migratory streams in the developing forebrain as seen by in situ hybridization at E13.5 and E15.5. A higher-magnification image of the cortex is shown beside each low-magnification panel of the forebrain. The upper panels show the expression of receptor genes in the PPL at E13.5 and MZ at E15.5. The lower panels show the expression of receptor genes predominantly in the IZ at E13.5 and E15.5. (A–B′) The expression of Reelin was used as an internal control, as it is known that it is expressed exclusively in cells (presumptive CR cells) in the PPL at E13.5 and in the MZ at E15.5. (C–J′) Expression of receptor genes Cnr1 (C–D′), Flrt2 (E–F′), Nelf (G–H′) and Ptpro (I–J) was localized predominantly within the PPL at E13.5 and within the MZ at E15.5. (K–L′) The interneuron marker Lhx6 was also used as an internal control, as it is known to be expressed in both the PPL and IZ at E13.5 (K–K′), and more widely, but predominantly in the MZ and IZ/SVZ, at E15.5 (L–L′). (M–R′) Expression of the receptor genes Cdh8 (M–N′), EphA3 (O–P′) and Neuritin (Q–R′) within the IZ at E13.5 and within the IZ/SVZ at E15.5. Scale bar in A–B′: 200 μm.
Figure 4: Expression of cell signalling genes in the interneuron migratory streams in the developing forebrain as seen by in situ hybridization at E13.5 and E15.5. A higher-magnification image of the cortex is shown beside each low-magnification panel of the forebrain. The upper panels show the expression of receptor genes in the PPL at E13.5 and in the MZ at E15.5. The lower panels show the expression of receptor genes predominantly in the IZ at E13.5 and E15.5. (A–B′) The expression of Reelin was used as an internal control, as it is known that it is expressed exclusively in cells (presumptive CR cells) in the PPL at E13.5 and in the MZ at E15.5. (C–D′) Expression of Dab1 is observed only within the PPL at E13.5 and in the MZ and SP (after the splitting of the CP) at E15.5. (E–F′) The interneuron marker Lhx6 was also used as an internal control, as it is known to be expressed in both the PPL and IZ at E13.5 (E–E′), and more widely, but predominantly in the MZ and IZ/SVZ, at E15.5 (F–F′). (G–L′) Expression of the cell signalling genes Cdc42ep3 (G–H′), Plcb1 (I–J′) and Rasgef1b (K–L′) was observed predominantly within the IZ at E13.5, and within the IZ/SVZ at E15.5. Scale bar in A–B′: 200 μm.

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Differential gene expression in migratory streams of cortical interneurons
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November 2011

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146 Reads

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45 Citations

Mary Antypa

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Clare Faux

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Gregor Eichele

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Cortical interneurons originate in the ganglionic eminences of the subpallium and migrate into the cortex in well-defined tangential streams. At the start of corticogenesis, two streams of migrating neurons are evident: a superficial one at the level of the preplate (PPL), and a deeper one at the level of the intermediate zone (IZ). Currently, little is known about the signalling mechanisms that regulate interneuron migration, and almost nothing is known about the molecules that may be involved in their choice of migratory stream. Here, we performed a microarray analysis, comparing the changes in gene expression between cells migrating in the PPL and those migrating in the IZ at embryonic day 13.5. This analysis identified genes, many of them novel, that were upregulated in one of the two streams. Moreover, polymerase chain reaction, in situ hybridization experiments and immunohistochemistry showed the expression of these genes in interneurons migrating within the PPL or IZ, suggesting that they play a role in their migration and choice of stream.

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Figure 1. Suppression of ARX protein expression by three shRNAs targeting different regions of ARX mRNA. A, Sequences of specific and triple-point-mutated shRNAs targeting mouse ARX mRNA. B, Representative confocal images of ARX protein expression in dissociated cell cultures of E16 rat ganglionic eminences transfected either with S2 or a control shRNA (DCX 3UTR3mhp). Each shRNA plasmid also encodes EGFP, enabling identification of transfected cells. Forty-eight hours after transfection, cells expressing the control shRNA were still immunopositive for ARX, whereas most cells transfected with ARX RNAi showed reduced ARX expression (arrows). C, COS-7 cells were transfected with an ARX-expressing plasmid and different shRNA constructs. Two days after transfection, cell lysates were subjected to Western blot analysis using ARX antibody. ARX levels in cells transfected with specific shRNAs (S1-S3) were significantly lower than those in cells transfected with triple-point-mutated shRNAs (S1m-S3m) or a control shRNA (DCX 3UTR3mhp).-Tubulin detection shows that similar amounts of proteins were loaded on the gel. D, Representative confocal images of ARX protein expression in COS-7 cells transfected with CMV-ARX and either S2 RNAi or a control RNAi (S2m or DCX 3UTR3mhp). E, Effect of the three shRNAs on ARX mRNA stability. COS-7 cells were transfected with psiCheck2ARX and different shRNAs. Forty-eight hours after transfection, Renilla and firefly luciferase activities were measured. The histogram shows Renilla luciferase data normalized to firefly luciferase measurements. Data represent the mean of 10 wells. Error bars indicate SEM. ***p 0.001, Student's t test. Scale bars: B, 20 m; D, 50 m.
Figure 2. Effect of ARX inactivation or overexpression on cell proliferation. A, B, Examination of E16.5 coronal sections of mouse brains electroporated at E13.5 with S2 shRNA or a control (S2m or DCX 3UTR3mhp) shRNA together with a DsRed-expressing vector. Sections were counterstained with 4,6-diamidino-2-phenylindole (DAPI). C, D, Brain sections were stained with an antibody that recognizes the mitotic marker P-H3 (blue). DsRed-positive cells labeled with P-H3 remain active in the cell cycle (arrows). E, F, Examination of E16.5 coronal sections of mouse brains electroporated at E13.5 with an ARX-overexpressing construct or an empty vector together with a DsRed plasmid. G, H, Brain sections were stained with antibodies against Ki67 or the mitotic marker P-H3 (blue). Scale bars, 30 m.
Figure 4. Disruption of radial migration in the neocortex after ARX silencing or overexpression. A-F, Examination of coronal sections of mouse brains electroporated at E13.5 with specific or control shRNAs. A-C, Three days after electroporation, cells expressing S2 shRNA were found primarily in the IZ (79.1 1.4% compared with 50.2 1.5% for S2m shRNA), with only a subset having reached the CP (14.7 1.2% compared with 35.1 1.4% for S2m shRNA). D-F, Although the effect of S1 shRNA on cell migration was less severe, there was an increased percentage of cells transfected with S1 in the deeper part of the CP (bins 6 and 7) and a subsequent decrease in the upper layers (bins 8 and 9) compared with the control. The limits of the CP are indicated by arrowheads. G-L, Examination of coronal sections of mouse brains electroporated at E13.5 with an empty vector or an ARX-overexpressing construct. G-I, By day 3, embryos electroporated with an ARX-overexpressing plasmid showed greater cell dispersion and fewer cells in the CP compared with controls (CAG-ARX: 38 2%, vs 57 1.4% for the control). J-L, By day 5, a large majority of control cells had reached the CP (76.9 1.4%). In contrast, only one-half of the cells expressing ARX were located in the CP (54.9 1.7%). Sections were counterstained with DAPI (4,6-diamidino-2-phenylindole; blue). Error bars indicate SEM. ***p 0.001, 2 test. Scale bars, 100 m.
Figure 5. Morphology of radially migrating neurons after ARX inactivation or overexpression in cortical progenitors. A-D, Morphology of cells in the SVZ/IZ of E16.5 mouse brains electroporated 3 d earlier with a specific (S2) or a control (S2m or DCX 3UTR3mhp) shRNA together with a DsRed-expressing plasmid. Many control cells migrated to the IZ and CP, where they became bipolar, whereas most ARX-inactivated cells in the IZ appeared round, showing very few or no processes (see insets). E-G, Examination of coronal sections of E16.5 mouse brains electroporated at E13.5 with an empty vector or an ARX-overexpressing construct. Tangentially orientated cells migrating away from the site of injection were detectable in the IZ of sections electroporated with ARX (see arrows). Some of these cells had long and complex processes, orientated tangentially (see insets). H, These cells represented 41.6 5.1% of the total number of cells with visible processes in the IZ, versus 0.9 1% for the control. I, J, Labeling of sections with anti-GABA antibody (blue) showed that none of these cells was GABA positive. Error bars indicate SEM. ***p 0.001, 2 test. Scale bars: A, B, E-G, 100 m; C, D, I, J, 50 m.
Figure 7. ARX does not control GABAergic cell specification. A1-A3, Colabeling ARX/GABA on E16 rat cortical sections. Some ARX-positive cells appear GABA (see arrows and insets). bv, Blood vessels. B1-B3, Colabeling ARX/GABA in dissociated E16 rat cortical cultures. Not all GABAergic cells express ARX (arrowheads). C1-C3, Colabeling ARX/GABA in dissociated E16 cultures from striatum. A few GABAergic cells negative for ARX (arrowheads) and some ARX-positive cells not expressing GABA (arrows) were observed. D, Quantification of the colocalization between ARX and GABA in dissociated E16 cultures from striatum kept for 3, 6, or 9 d in vitro. E, ARX overexpression does not induce GABA or calbindin expression in rat E16 dissociated cultures from cortex or GE. F, Percentage of GFP cells expressing GABA or calbindin after transfection with CAG-ARX or the vector alone. Scale bars: A1-A3, 100 m; B1-C3, E, 40 m.
Cell-Autonomous Roles of ARX in Cell Proliferation and Neuronal Migration during Corticogenesis

June 2008

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223 Reads

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122 Citations

The Journal of Neuroscience : The Official Journal of the Society for Neuroscience

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Shigeaki Kanatani

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John G Parnavelas

The aristaless-related homeobox (ARX) gene has been implicated in a wide spectrum of disorders ranging from phenotypes with severe neuronal migration defects, such as lissencephaly, to mild forms of X-linked mental retardation without apparent brain abnormalities. To better understand its role in corticogenesis, we used in utero electroporation to knock down or overexpress ARX. We show here that targeted inhibition of ARX causes cortical progenitor cells to exit the cell cycle prematurely and impairs their migration toward the cortical plate. In contrast, ARX overexpression increases the length of the cell cycle. In addition, we report that RNA interference-mediated inactivation of ARX prevents cells from acquiring multipolar morphology in the subventricular and intermediate zones, resulting in decreased neuronal motility. In contrast, ARX overexpression appears to promote the development of tangentially oriented processes of cells in the subventricular and intermediate zones and affects radial migration of pyramidal neurons. We also demonstrate that the level of ARX expression is important for tangential migration of GABA-containing interneurons, because both inactivation and overexpression of the gene impair their migration from the ganglionic eminence. However, our data suggest that ARX is not directly involved in GABAergic cell fate specification. Overall, these results identify multiple and distinct cell-autonomous roles for ARX in corticogenesis.

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Figure 1. DCX protein expression in embryonic rat forebrain and DCX silencing using RNAi. A, DCX expression in a coronal section through an E16 rat brain. Labeling was abundant throughout the cortical mantle, including a stream of horizontally oriented cells at the level of the lower IZ and a small number of cells in the VZ. A1–A3 (boxed area in A), Double-labeling showed that many of the DCX cells in these zones were also positive for GABA. B, Representative confocal images of DCX protein expression in dissociated cortical cells transfected with either DCX or a control RNAi (3UTR3mhp). Each shRNA plasmid also encodes GFP, enabling identification of transfected cells. Forty-eight hours after transfection, cells expressing the control shRNA were still immunopositive for DCX, whereas most of the cells transfected with DCX RNAi were DCX deficient. DAPI, 4,6-Diamidino-2- phenylindole. C, After injection and focal electroporation with either DCX RNAi or a control RNAi together with CAG-IRES-EGFP, brain slices were immunolabeled using DCX antibody. A large majority of the cells transfected with DCX RNAi were negative for DCX labeling, further demonstrating the efficacy of the shRNA. D, COS-7 cells were transfected with a DCX-expressing plasmid and with either DCX RNAi or a control RNAi. Two days after transfection, cell lysates were subjected to Western blot analysis using DCX antibody. -Tubulin detection shows that similar amounts of proteins were loaded on the gel. Scale bars: A, 100 m; B, C,20m.  
Figure 2. Effect of DCX RNAi on interneuron migration and morphology. A, The ganglionic eminence in an E17 rat brain slice was injected and focally electroporated with either DCX RNAi or a control RNAi (3UTR3mhp) together with CAG-IRES-EGFP. Cells transfected with DCX RNAi still migrated to the cortex, but were reduced in number. B, The cortex was divided into three sectors (I–III), and the number of GFP cells was counted in each sector. The result was expressed as a percentage of cells detected in each sector divided by the total number of cells that migrated into the cortex. The vast majority of DCX-silenced cells were located in sector I, whereas control cells were more spread in the three sectors (28 and 25 sections analyzed for DCX RNAi and the control, respectively). ***p 0.001, 2 test. C, The ganglionic eminence of an E17 rat brain slice was injected with DCX RNAi and either CAG-IRES-EGFP vector alone or CAG-DCX (n 15 sections analyzed for both). In the presence of the rescue construct, there was a significant decrease of the number of cells in sector I of the cortex combined with an increase in cell numbers in sectors II and III. ***p 0.001; **p 0.01, 2 test. D, Morphology of the DCX-inactivated cells. Representative confocal images of GFP-positive cells migrating into the cortex of embryonic rat brain slices show a higher complexity of branching in DCX-silenced cells. E, The number of primary processes arising from the cell bodies and total branches were counted for GFP-positive cells migrating tangentially in the cortex (n 48 cells from 14 sections for DCX RNAi and n 77 cells from 16 sections for the control RNAi). The histogram illustrates that, although the numbers of primary processes were similar in the two groups of cells, those inactivated for DCX tended to have more branches than control cells. ***p 0.001; *p 0.05, Student's t test. F, Rescue of the branching defect after coelectroporation of either DCX RNAi and the CAG vector alone (n 44 cells from 10 sections) or DCX RNAi and CAG-DCX plasmids (n 11 cells from 4 sections). Scale bars: A, 100 m; D, 15 m. Error bars indicate SEM.  
Figure 3. DCLK and DCX are both necessary for proper interneuron migration. A, Rat E16 cortical cell cultures were transfected with DCLK shRNA, a mutated DCLK shRNA, or DCX shRNA and labeled using antibodies directed against DCLK or DCX. DCLK RNAi led to specific knock-down of DCLK, whereas DCX RNAi did not have any effect on DCLK expression. Similarly, DCX RNAi had a specific effect on DCX expression. B, Electroporation of DCLK RNAi in the GE of E17 rat brain slices. As previously, the cortex was divided into three sectors and the number of cells were counted in each (22 and 38 sections analyzed for DCLK RNAi and control, respectively). Similar to DCX RNAi, there was a significant increase in the proportion of cells in sector I of the cortex combined with a decrease in sectors II and III. **p 0.01; *p 0.05, 2 test. C, Electroporation of both DCX and DCLK shRNAs together led to even less migration in the cortex compared with controls (3UTR3mhp and DCLKm). D, No branching defect was found to be associated with DCLK RNAi. As previously, the number of primary processes and total branching were counted for GFP cells migrating tangentially into the cortex (n 42 cells from 8 sections for DCLK RNAi alone; n 55 cells from 11 sections for DCX/DCLK RNAi; n 56 cells from 18 sections for the control). The histogram shows that, although the number of primary processes or total branching for DCLK RNAi was not different from the control, the combined DCX/DCLK shRNAs showed increased branching, similar to DCX RNAi alone. Scale bars: A, 10 m; C, 40 m. Error bars indicate SEM.  
Figure 4. Interneuron defects in Dcx, Dclk, and Dcx/Dclk mutant mice. A–H, Calbindin labeling in coronal sections from P0 mutant animals. I, Quantification of the number of calbindin-positive cells in the cortex of mutant mice. The histogram depicts the average number of calbindin-positive cells in a 200-m-wide radial strip of dorsal and lateral cortex in wild-type and mutant brain sections at P0. All three genotypes show a significantly decreased number of calbindin-positive cells in the cortex. ***p 0.001, Student's t test. J1–J3, The cortical plate (a 400-m-wide radial strip) at dorsomedial level was divided into 10 equally spaced bins (as shown in H ). The number of cells in each bin was expressed as a percentage of the total number of cells. For each genotype, the distribution was different from the wild-type. ***p 0.001; **p 0.01; *p 0.05, 2 test. Scale bars: A–D, 400 m; B–H, 200 m. Error bars indicate SEM.  
Both Doublecortin and Doublecortin-Like Kinase Play a Role in Cortical Interneuron Migration

May 2007

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645 Reads

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147 Citations

The Journal of Neuroscience : The Official Journal of the Society for Neuroscience

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Mary Antypa

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John G Parnavelas

Type I lissencephaly, a genetic disease characterized by disorganized cortical layers and gyral abnormalities, is associated with severe cognitive impairment and epilepsy. Two genes, LIS1 and doublecortin (DCX), have been shown to be responsible for a large proportion of cases of type I lissencephaly. Both genes encode microtubule-associated proteins that have been shown to be important for radial migration of cortical pyramidal neurons. To investigate whether DCX also plays a role in cortical interneuron migration, we inactivated DCX in the ganglionic eminence of rat embryonic day 17 brain slices using short hairpin RNA. We found that, when DCX expression was blocked, the migration of interneurons from the ganglionic eminence to the cerebral cortex was slowed but not absent, similar to what had previously been reported for radial neuronal migration. In addition, the processes of DCX-deficient migrating interneurons were more branched than their counterparts in control experiments. These effects were rescued by DCX overexpression, confirming the specificity to DCX inactivation. A similar delay in interneuron migration was observed when Doublecortin-like kinase (DCLK), a microtubule-associated protein related to DCX, was inactivated, although the morphology of the cells was not affected. The importance of these genes in interneuron migration was confirmed by our finding that the cortices of Dcx, Dclk, and Dcx/Dclk mutant mice contained a reduced number of such cells in the cortex and their distribution was different compared with wild-type controls. However, the defect was different for each group of mutant animals, suggesting that DCX and DCLK have distinct roles in cortical interneuron migration.

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Citations (3)

... Cell-to-cell contacts modulate this complex intercommunication through a gradient of different molecules called morphogens. Morphogens are secreted during the proliferation of neural progenitor cells and determine the programmed movement and distribution of neural and glial progenies resulting from the proliferation, distribution, and migration of these cell lineages during the formation of the cerebral cortex, cerebellum, and spinal cord [38,39]. Several lipidrelated molecules, such as sphingolipids, glycolipids, phospholipids, thromboxanes, and prostaglandins, constitute these bioactive signals and are crucial for synaptic differentiation and plasticity [40]. ...

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Modeling the Effect of Cannabinoid Exposure During Human Neurodevelopment Using Bidimensional and Tridimensional Cultures
Differential gene expression in migratory streams of cortical interneurons
Mary Antypa

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Clare Faux

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Gregor Eichele

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... Beyond the regulation of actin cytoskeleton components, our results also show a reduction in DCX, suggesting a potential disruption in microtubule dynamics. In agreement with our findings, DCX knockout has been linked to slowed interneuron migration and branching defects [112,113]. While previous studies report varied migration dynamics, they both support the notion that reduced DCX expression leads to abnormal interneuron migration, aligning with our findings. ...

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Interneuron migration impairment and brain region-specific DNA damage response following irradiation during early neurogenesis in mice
Both Doublecortin and Doublecortin-Like Kinase Play a Role in Cortical Interneuron Migration

The Journal of Neuroscience : The Official Journal of the Society for Neuroscience

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Mary Antypa

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John G Parnavelas

... The aristaless homeobox, Arx, gene is one such factor but due to high expression in other cell types could not be assessed reliably via western blots. In addition to being regulated by LHX6 and DLX proteins (Colasante et al., 2008;Vogt et al., 2014;Zhao et al., 2008), it also controls CIN developmental properties (Friocourt et al., 2008;Joseph et al., 2021, 202;Marsh et al., 2016;Ruggieri et al., 2010). We examined E15.5 brains for ARX expression and found a 31% and 44% reduction in Nf1 cKO and bRaf ca brains, respectively We also assessed an equivalent age for WT and bRaf ca MGE transplanted cells. ...

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Distinct hyperactive RAS/MAPK alleles converge on common GABAergic interneuron core programs
Cell-Autonomous Roles of ARX in Cell Proliferation and Neuronal Migration during Corticogenesis

The Journal of Neuroscience : The Official Journal of the Society for Neuroscience

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Shigeaki Kanatani

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John G Parnavelas