scale tool Search Results


genomic scale data visualization tool  (Golden Helix)
90
Golden Helix genomic scale data visualization tool
Genomic Scale Data Visualization Tool, supplied by Golden Helix, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/result/genomic scale data visualization tool/product/Golden Helix
Average 90 stars, based on 1 article reviews
genomic scale data visualization tool - by Bioz Stars, 2026-04
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internal scaling tool  (OpenSim Ltd)
90
OpenSim Ltd internal scaling tool
Internal Scaling Tool, supplied by OpenSim Ltd, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/result/internal scaling tool/product/OpenSim Ltd
Average 90 stars, based on 1 article reviews
internal scaling tool - by Bioz Stars, 2026-04
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opensim scaling  (OpenSim Ltd)
90
OpenSim Ltd opensim scaling
Opensim Scaling, supplied by OpenSim Ltd, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/result/opensim scaling/product/OpenSim Ltd
Average 90 stars, based on 1 article reviews
opensim scaling - by Bioz Stars, 2026-04
90/100 stars
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scale tool  (OpenSim Ltd)
90
OpenSim Ltd scale tool
Scale Tool, supplied by OpenSim Ltd, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/result/scale tool/product/OpenSim Ltd
Average 90 stars, based on 1 article reviews
scale tool - by Bioz Stars, 2026-04
90/100 stars
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micro or mesoscale machine tool 640  (Meso Scale Diagnostics LLC)
90
Meso Scale Diagnostics LLC micro or mesoscale machine tool 640
Micro Or Mesoscale Machine Tool 640, supplied by Meso Scale Diagnostics LLC, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/result/micro or mesoscale machine tool 640/product/Meso Scale Diagnostics LLC
Average 90 stars, based on 1 article reviews
micro or mesoscale machine tool 640 - by Bioz Stars, 2026-04
90/100 stars
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processing and imaging tool kit  (Small Scale Industries)
90
Small Scale Industries processing and imaging tool kit
Processing And Imaging Tool Kit, supplied by Small Scale Industries, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/result/processing and imaging tool kit/product/Small Scale Industries
Average 90 stars, based on 1 article reviews
processing and imaging tool kit - by Bioz Stars, 2026-04
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2d scale tool  (Amira Pharmaceuticals)
90
Amira Pharmaceuticals 2d scale tool
Pronuclear membranes persist after prophase and become highly fenestrated in metaphase. (A and B) A one-cell embryo expressing the NE protein LEM-2 fused to GFP and histone H2B fused to mCherry was imaged at the indicated time points (metaphase = time 0). LEM-2 persists on the pronuclear membranes throughout mitosis, allowing the visualization of the pronuclear membranes between the two pronuclei. Merging of parental chromosome occurs at metaphase through a fenestration in the pronuclear interface membranes (B). Scale bars, 10 µm. (C) <t>2D</t> cross sections from FIB-SEM image volumes of a subset of embryos (top row) and their reconstructed chromosomes (middle row) used in this study. The illustration on the left depicts the orientation of the centrosomes (orange circle) and spindle microtubules (black lines) relative to the images shown (chromosomes are in red). Some panels are from the plane of imaging and some are oblique 2D slices through a reconstructed FIB-SEM image volume, aligned orthogonal to the membrane interface. Embryos were ordered from prometaphase to metaphase by the degree of chromosome alignment and compaction, based on total chromosome volumes, shown below <t>the</t> <t>3D</t> chromosome reconstructions. The pronuclei shown are from the following embryos (from left to right): PM2, PM4, M1, M2, and M3. Scale bars, 1 µm. (D) Examples of peripheral pronuclear membranes (blue rectangle in the cartoon depiction of two associated pronuclei) from prophase (P1), prometaphase (PM2), and metaphase (M1) embryos. The image on the far left is an enlargement of a membrane segment from the prometaphase embryos showing the two nuclear membranes (inner and outer) and the constriction that is seen where an NPC is embedded. Arrowheads in the “metaphase” panel point to holes that are larger than the expected size for NPC holes. Scale bars represent 500 nm, except in the inset, where the scale bar represents 100 nm. INM, inner nuclear membrane; ONM, outer nuclear membrane. (E) Segmented volumes of peripheral pronuclear membranes from the embryos shown in D. Scale bars represent 500 nm, except for the metaphase image on the right, for which the scale bar is 1 µm. P1, prophase; PM2, prometaphase; M1, metaphase. (F) Quantification of hole area in the peripheral pronuclear membranes of an embryo in prophase (P; embryo P1), prometaphase (PM; embryo PM2) and two embryos in metaphase (M1 and M2). For each embryo, data were derived from several segmented areas that were at least 1 µm 2 in size. The total number of holes measured and number of areas per embryo were as follows: prophase, n = 213, nine areas; prometaphase, n = 153, nine areas; M1, n = 58, six areas; and M2, n = 46, five areas. Note that the y axis is discontinuous; blue background highlights the upper segment of the graph (hole area >0.04 µm 2 ). Statistical analyses were done using the Kruskal-Wallis test with correction for multiple comparisons. The adjusted P values for the nonsignificant differences (n.s.) were >0.9999. See for statistical analyses of the lower segment.
2d Scale Tool, supplied by Amira Pharmaceuticals, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/result/2d scale tool/product/Amira Pharmaceuticals
Average 90 stars, based on 1 article reviews
2d scale tool - by Bioz Stars, 2026-04
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nano-scale electrical contact resistance tool nanoecr  (Bruker Corporation)
90
Bruker Corporation nano-scale electrical contact resistance tool nanoecr
Pronuclear membranes persist after prophase and become highly fenestrated in metaphase. (A and B) A one-cell embryo expressing the NE protein LEM-2 fused to GFP and histone H2B fused to mCherry was imaged at the indicated time points (metaphase = time 0). LEM-2 persists on the pronuclear membranes throughout mitosis, allowing the visualization of the pronuclear membranes between the two pronuclei. Merging of parental chromosome occurs at metaphase through a fenestration in the pronuclear interface membranes (B). Scale bars, 10 µm. (C) <t>2D</t> cross sections from FIB-SEM image volumes of a subset of embryos (top row) and their reconstructed chromosomes (middle row) used in this study. The illustration on the left depicts the orientation of the centrosomes (orange circle) and spindle microtubules (black lines) relative to the images shown (chromosomes are in red). Some panels are from the plane of imaging and some are oblique 2D slices through a reconstructed FIB-SEM image volume, aligned orthogonal to the membrane interface. Embryos were ordered from prometaphase to metaphase by the degree of chromosome alignment and compaction, based on total chromosome volumes, shown below <t>the</t> <t>3D</t> chromosome reconstructions. The pronuclei shown are from the following embryos (from left to right): PM2, PM4, M1, M2, and M3. Scale bars, 1 µm. (D) Examples of peripheral pronuclear membranes (blue rectangle in the cartoon depiction of two associated pronuclei) from prophase (P1), prometaphase (PM2), and metaphase (M1) embryos. The image on the far left is an enlargement of a membrane segment from the prometaphase embryos showing the two nuclear membranes (inner and outer) and the constriction that is seen where an NPC is embedded. Arrowheads in the “metaphase” panel point to holes that are larger than the expected size for NPC holes. Scale bars represent 500 nm, except in the inset, where the scale bar represents 100 nm. INM, inner nuclear membrane; ONM, outer nuclear membrane. (E) Segmented volumes of peripheral pronuclear membranes from the embryos shown in D. Scale bars represent 500 nm, except for the metaphase image on the right, for which the scale bar is 1 µm. P1, prophase; PM2, prometaphase; M1, metaphase. (F) Quantification of hole area in the peripheral pronuclear membranes of an embryo in prophase (P; embryo P1), prometaphase (PM; embryo PM2) and two embryos in metaphase (M1 and M2). For each embryo, data were derived from several segmented areas that were at least 1 µm 2 in size. The total number of holes measured and number of areas per embryo were as follows: prophase, n = 213, nine areas; prometaphase, n = 153, nine areas; M1, n = 58, six areas; and M2, n = 46, five areas. Note that the y axis is discontinuous; blue background highlights the upper segment of the graph (hole area >0.04 µm 2 ). Statistical analyses were done using the Kruskal-Wallis test with correction for multiple comparisons. The adjusted P values for the nonsignificant differences (n.s.) were >0.9999. See for statistical analyses of the lower segment.
Nano Scale Electrical Contact Resistance Tool Nanoecr, supplied by Bruker Corporation, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/result/nano-scale electrical contact resistance tool nanoecr/product/Bruker Corporation
Average 90 stars, based on 1 article reviews
nano-scale electrical contact resistance tool nanoecr - by Bioz Stars, 2026-04
90/100 stars
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ball bearing tool with vernier scale  (Elekta)
90
Elekta ball bearing tool with vernier scale
Pronuclear membranes persist after prophase and become highly fenestrated in metaphase. (A and B) A one-cell embryo expressing the NE protein LEM-2 fused to GFP and histone H2B fused to mCherry was imaged at the indicated time points (metaphase = time 0). LEM-2 persists on the pronuclear membranes throughout mitosis, allowing the visualization of the pronuclear membranes between the two pronuclei. Merging of parental chromosome occurs at metaphase through a fenestration in the pronuclear interface membranes (B). Scale bars, 10 µm. (C) <t>2D</t> cross sections from FIB-SEM image volumes of a subset of embryos (top row) and their reconstructed chromosomes (middle row) used in this study. The illustration on the left depicts the orientation of the centrosomes (orange circle) and spindle microtubules (black lines) relative to the images shown (chromosomes are in red). Some panels are from the plane of imaging and some are oblique 2D slices through a reconstructed FIB-SEM image volume, aligned orthogonal to the membrane interface. Embryos were ordered from prometaphase to metaphase by the degree of chromosome alignment and compaction, based on total chromosome volumes, shown below <t>the</t> <t>3D</t> chromosome reconstructions. The pronuclei shown are from the following embryos (from left to right): PM2, PM4, M1, M2, and M3. Scale bars, 1 µm. (D) Examples of peripheral pronuclear membranes (blue rectangle in the cartoon depiction of two associated pronuclei) from prophase (P1), prometaphase (PM2), and metaphase (M1) embryos. The image on the far left is an enlargement of a membrane segment from the prometaphase embryos showing the two nuclear membranes (inner and outer) and the constriction that is seen where an NPC is embedded. Arrowheads in the “metaphase” panel point to holes that are larger than the expected size for NPC holes. Scale bars represent 500 nm, except in the inset, where the scale bar represents 100 nm. INM, inner nuclear membrane; ONM, outer nuclear membrane. (E) Segmented volumes of peripheral pronuclear membranes from the embryos shown in D. Scale bars represent 500 nm, except for the metaphase image on the right, for which the scale bar is 1 µm. P1, prophase; PM2, prometaphase; M1, metaphase. (F) Quantification of hole area in the peripheral pronuclear membranes of an embryo in prophase (P; embryo P1), prometaphase (PM; embryo PM2) and two embryos in metaphase (M1 and M2). For each embryo, data were derived from several segmented areas that were at least 1 µm 2 in size. The total number of holes measured and number of areas per embryo were as follows: prophase, n = 213, nine areas; prometaphase, n = 153, nine areas; M1, n = 58, six areas; and M2, n = 46, five areas. Note that the y axis is discontinuous; blue background highlights the upper segment of the graph (hole area >0.04 µm 2 ). Statistical analyses were done using the Kruskal-Wallis test with correction for multiple comparisons. The adjusted P values for the nonsignificant differences (n.s.) were >0.9999. See for statistical analyses of the lower segment.
Ball Bearing Tool With Vernier Scale, supplied by Elekta, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/result/ball bearing tool with vernier scale/product/Elekta
Average 90 stars, based on 1 article reviews
ball bearing tool with vernier scale - by Bioz Stars, 2026-04
90/100 stars
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optical tool  (Meso Scale Diagnostics LLC)
90
Meso Scale Diagnostics LLC optical tool
Pronuclear membranes persist after prophase and become highly fenestrated in metaphase. (A and B) A one-cell embryo expressing the NE protein LEM-2 fused to GFP and histone H2B fused to mCherry was imaged at the indicated time points (metaphase = time 0). LEM-2 persists on the pronuclear membranes throughout mitosis, allowing the visualization of the pronuclear membranes between the two pronuclei. Merging of parental chromosome occurs at metaphase through a fenestration in the pronuclear interface membranes (B). Scale bars, 10 µm. (C) <t>2D</t> cross sections from FIB-SEM image volumes of a subset of embryos (top row) and their reconstructed chromosomes (middle row) used in this study. The illustration on the left depicts the orientation of the centrosomes (orange circle) and spindle microtubules (black lines) relative to the images shown (chromosomes are in red). Some panels are from the plane of imaging and some are oblique 2D slices through a reconstructed FIB-SEM image volume, aligned orthogonal to the membrane interface. Embryos were ordered from prometaphase to metaphase by the degree of chromosome alignment and compaction, based on total chromosome volumes, shown below <t>the</t> <t>3D</t> chromosome reconstructions. The pronuclei shown are from the following embryos (from left to right): PM2, PM4, M1, M2, and M3. Scale bars, 1 µm. (D) Examples of peripheral pronuclear membranes (blue rectangle in the cartoon depiction of two associated pronuclei) from prophase (P1), prometaphase (PM2), and metaphase (M1) embryos. The image on the far left is an enlargement of a membrane segment from the prometaphase embryos showing the two nuclear membranes (inner and outer) and the constriction that is seen where an NPC is embedded. Arrowheads in the “metaphase” panel point to holes that are larger than the expected size for NPC holes. Scale bars represent 500 nm, except in the inset, where the scale bar represents 100 nm. INM, inner nuclear membrane; ONM, outer nuclear membrane. (E) Segmented volumes of peripheral pronuclear membranes from the embryos shown in D. Scale bars represent 500 nm, except for the metaphase image on the right, for which the scale bar is 1 µm. P1, prophase; PM2, prometaphase; M1, metaphase. (F) Quantification of hole area in the peripheral pronuclear membranes of an embryo in prophase (P; embryo P1), prometaphase (PM; embryo PM2) and two embryos in metaphase (M1 and M2). For each embryo, data were derived from several segmented areas that were at least 1 µm 2 in size. The total number of holes measured and number of areas per embryo were as follows: prophase, n = 213, nine areas; prometaphase, n = 153, nine areas; M1, n = 58, six areas; and M2, n = 46, five areas. Note that the y axis is discontinuous; blue background highlights the upper segment of the graph (hole area >0.04 µm 2 ). Statistical analyses were done using the Kruskal-Wallis test with correction for multiple comparisons. The adjusted P values for the nonsignificant differences (n.s.) were >0.9999. See for statistical analyses of the lower segment.
Optical Tool, supplied by Meso Scale Diagnostics LLC, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/result/optical tool/product/Meso Scale Diagnostics LLC
Average 90 stars, based on 1 article reviews
optical tool - by Bioz Stars, 2026-04
90/100 stars
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scale bar tool  (Amira Pharmaceuticals)
90
Amira Pharmaceuticals scale bar tool
Pronuclear membranes persist after prophase and become highly fenestrated in metaphase. (A and B) A one-cell embryo expressing the NE protein LEM-2 fused to GFP and histone H2B fused to mCherry was imaged at the indicated time points (metaphase = time 0). LEM-2 persists on the pronuclear membranes throughout mitosis, allowing the visualization of the pronuclear membranes between the two pronuclei. Merging of parental chromosome occurs at metaphase through a fenestration in the pronuclear interface membranes (B). Scale bars, 10 µm. (C) <t>2D</t> cross sections from FIB-SEM image volumes of a subset of embryos (top row) and their reconstructed chromosomes (middle row) used in this study. The illustration on the left depicts the orientation of the centrosomes (orange circle) and spindle microtubules (black lines) relative to the images shown (chromosomes are in red). Some panels are from the plane of imaging and some are oblique 2D slices through a reconstructed FIB-SEM image volume, aligned orthogonal to the membrane interface. Embryos were ordered from prometaphase to metaphase by the degree of chromosome alignment and compaction, based on total chromosome volumes, shown below <t>the</t> <t>3D</t> chromosome reconstructions. The pronuclei shown are from the following embryos (from left to right): PM2, PM4, M1, M2, and M3. Scale bars, 1 µm. (D) Examples of peripheral pronuclear membranes (blue rectangle in the cartoon depiction of two associated pronuclei) from prophase (P1), prometaphase (PM2), and metaphase (M1) embryos. The image on the far left is an enlargement of a membrane segment from the prometaphase embryos showing the two nuclear membranes (inner and outer) and the constriction that is seen where an NPC is embedded. Arrowheads in the “metaphase” panel point to holes that are larger than the expected size for NPC holes. Scale bars represent 500 nm, except in the inset, where the scale bar represents 100 nm. INM, inner nuclear membrane; ONM, outer nuclear membrane. (E) Segmented volumes of peripheral pronuclear membranes from the embryos shown in D. Scale bars represent 500 nm, except for the metaphase image on the right, for which the scale bar is 1 µm. P1, prophase; PM2, prometaphase; M1, metaphase. (F) Quantification of hole area in the peripheral pronuclear membranes of an embryo in prophase (P; embryo P1), prometaphase (PM; embryo PM2) and two embryos in metaphase (M1 and M2). For each embryo, data were derived from several segmented areas that were at least 1 µm 2 in size. The total number of holes measured and number of areas per embryo were as follows: prophase, n = 213, nine areas; prometaphase, n = 153, nine areas; M1, n = 58, six areas; and M2, n = 46, five areas. Note that the y axis is discontinuous; blue background highlights the upper segment of the graph (hole area >0.04 µm 2 ). Statistical analyses were done using the Kruskal-Wallis test with correction for multiple comparisons. The adjusted P values for the nonsignificant differences (n.s.) were >0.9999. See for statistical analyses of the lower segment.
Scale Bar Tool, supplied by Amira Pharmaceuticals, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/result/scale bar tool/product/Amira Pharmaceuticals
Average 90 stars, based on 1 article reviews
scale bar tool - by Bioz Stars, 2026-04
90/100 stars
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scale tool  (JENOPTIK Inc)
90
JENOPTIK Inc scale tool
Pronuclear membranes persist after prophase and become highly fenestrated in metaphase. (A and B) A one-cell embryo expressing the NE protein LEM-2 fused to GFP and histone H2B fused to mCherry was imaged at the indicated time points (metaphase = time 0). LEM-2 persists on the pronuclear membranes throughout mitosis, allowing the visualization of the pronuclear membranes between the two pronuclei. Merging of parental chromosome occurs at metaphase through a fenestration in the pronuclear interface membranes (B). Scale bars, 10 µm. (C) <t>2D</t> cross sections from FIB-SEM image volumes of a subset of embryos (top row) and their reconstructed chromosomes (middle row) used in this study. The illustration on the left depicts the orientation of the centrosomes (orange circle) and spindle microtubules (black lines) relative to the images shown (chromosomes are in red). Some panels are from the plane of imaging and some are oblique 2D slices through a reconstructed FIB-SEM image volume, aligned orthogonal to the membrane interface. Embryos were ordered from prometaphase to metaphase by the degree of chromosome alignment and compaction, based on total chromosome volumes, shown below <t>the</t> <t>3D</t> chromosome reconstructions. The pronuclei shown are from the following embryos (from left to right): PM2, PM4, M1, M2, and M3. Scale bars, 1 µm. (D) Examples of peripheral pronuclear membranes (blue rectangle in the cartoon depiction of two associated pronuclei) from prophase (P1), prometaphase (PM2), and metaphase (M1) embryos. The image on the far left is an enlargement of a membrane segment from the prometaphase embryos showing the two nuclear membranes (inner and outer) and the constriction that is seen where an NPC is embedded. Arrowheads in the “metaphase” panel point to holes that are larger than the expected size for NPC holes. Scale bars represent 500 nm, except in the inset, where the scale bar represents 100 nm. INM, inner nuclear membrane; ONM, outer nuclear membrane. (E) Segmented volumes of peripheral pronuclear membranes from the embryos shown in D. Scale bars represent 500 nm, except for the metaphase image on the right, for which the scale bar is 1 µm. P1, prophase; PM2, prometaphase; M1, metaphase. (F) Quantification of hole area in the peripheral pronuclear membranes of an embryo in prophase (P; embryo P1), prometaphase (PM; embryo PM2) and two embryos in metaphase (M1 and M2). For each embryo, data were derived from several segmented areas that were at least 1 µm 2 in size. The total number of holes measured and number of areas per embryo were as follows: prophase, n = 213, nine areas; prometaphase, n = 153, nine areas; M1, n = 58, six areas; and M2, n = 46, five areas. Note that the y axis is discontinuous; blue background highlights the upper segment of the graph (hole area >0.04 µm 2 ). Statistical analyses were done using the Kruskal-Wallis test with correction for multiple comparisons. The adjusted P values for the nonsignificant differences (n.s.) were >0.9999. See for statistical analyses of the lower segment.
Scale Tool, supplied by JENOPTIK Inc, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/result/scale tool/product/JENOPTIK Inc
Average 90 stars, based on 1 article reviews
scale tool - by Bioz Stars, 2026-04
90/100 stars
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Image Search Results


Pronuclear membranes persist after prophase and become highly fenestrated in metaphase. (A and B) A one-cell embryo expressing the NE protein LEM-2 fused to GFP and histone H2B fused to mCherry was imaged at the indicated time points (metaphase = time 0). LEM-2 persists on the pronuclear membranes throughout mitosis, allowing the visualization of the pronuclear membranes between the two pronuclei. Merging of parental chromosome occurs at metaphase through a fenestration in the pronuclear interface membranes (B). Scale bars, 10 µm. (C) 2D cross sections from FIB-SEM image volumes of a subset of embryos (top row) and their reconstructed chromosomes (middle row) used in this study. The illustration on the left depicts the orientation of the centrosomes (orange circle) and spindle microtubules (black lines) relative to the images shown (chromosomes are in red). Some panels are from the plane of imaging and some are oblique 2D slices through a reconstructed FIB-SEM image volume, aligned orthogonal to the membrane interface. Embryos were ordered from prometaphase to metaphase by the degree of chromosome alignment and compaction, based on total chromosome volumes, shown below the 3D chromosome reconstructions. The pronuclei shown are from the following embryos (from left to right): PM2, PM4, M1, M2, and M3. Scale bars, 1 µm. (D) Examples of peripheral pronuclear membranes (blue rectangle in the cartoon depiction of two associated pronuclei) from prophase (P1), prometaphase (PM2), and metaphase (M1) embryos. The image on the far left is an enlargement of a membrane segment from the prometaphase embryos showing the two nuclear membranes (inner and outer) and the constriction that is seen where an NPC is embedded. Arrowheads in the “metaphase” panel point to holes that are larger than the expected size for NPC holes. Scale bars represent 500 nm, except in the inset, where the scale bar represents 100 nm. INM, inner nuclear membrane; ONM, outer nuclear membrane. (E) Segmented volumes of peripheral pronuclear membranes from the embryos shown in D. Scale bars represent 500 nm, except for the metaphase image on the right, for which the scale bar is 1 µm. P1, prophase; PM2, prometaphase; M1, metaphase. (F) Quantification of hole area in the peripheral pronuclear membranes of an embryo in prophase (P; embryo P1), prometaphase (PM; embryo PM2) and two embryos in metaphase (M1 and M2). For each embryo, data were derived from several segmented areas that were at least 1 µm 2 in size. The total number of holes measured and number of areas per embryo were as follows: prophase, n = 213, nine areas; prometaphase, n = 153, nine areas; M1, n = 58, six areas; and M2, n = 46, five areas. Note that the y axis is discontinuous; blue background highlights the upper segment of the graph (hole area >0.04 µm 2 ). Statistical analyses were done using the Kruskal-Wallis test with correction for multiple comparisons. The adjusted P values for the nonsignificant differences (n.s.) were >0.9999. See for statistical analyses of the lower segment.

Journal: The Journal of Cell Biology

Article Title: C. elegans pronuclei fuse after fertilization through a novel membrane structure

doi: 10.1083/jcb.201909137

Figure Lengend Snippet: Pronuclear membranes persist after prophase and become highly fenestrated in metaphase. (A and B) A one-cell embryo expressing the NE protein LEM-2 fused to GFP and histone H2B fused to mCherry was imaged at the indicated time points (metaphase = time 0). LEM-2 persists on the pronuclear membranes throughout mitosis, allowing the visualization of the pronuclear membranes between the two pronuclei. Merging of parental chromosome occurs at metaphase through a fenestration in the pronuclear interface membranes (B). Scale bars, 10 µm. (C) 2D cross sections from FIB-SEM image volumes of a subset of embryos (top row) and their reconstructed chromosomes (middle row) used in this study. The illustration on the left depicts the orientation of the centrosomes (orange circle) and spindle microtubules (black lines) relative to the images shown (chromosomes are in red). Some panels are from the plane of imaging and some are oblique 2D slices through a reconstructed FIB-SEM image volume, aligned orthogonal to the membrane interface. Embryos were ordered from prometaphase to metaphase by the degree of chromosome alignment and compaction, based on total chromosome volumes, shown below the 3D chromosome reconstructions. The pronuclei shown are from the following embryos (from left to right): PM2, PM4, M1, M2, and M3. Scale bars, 1 µm. (D) Examples of peripheral pronuclear membranes (blue rectangle in the cartoon depiction of two associated pronuclei) from prophase (P1), prometaphase (PM2), and metaphase (M1) embryos. The image on the far left is an enlargement of a membrane segment from the prometaphase embryos showing the two nuclear membranes (inner and outer) and the constriction that is seen where an NPC is embedded. Arrowheads in the “metaphase” panel point to holes that are larger than the expected size for NPC holes. Scale bars represent 500 nm, except in the inset, where the scale bar represents 100 nm. INM, inner nuclear membrane; ONM, outer nuclear membrane. (E) Segmented volumes of peripheral pronuclear membranes from the embryos shown in D. Scale bars represent 500 nm, except for the metaphase image on the right, for which the scale bar is 1 µm. P1, prophase; PM2, prometaphase; M1, metaphase. (F) Quantification of hole area in the peripheral pronuclear membranes of an embryo in prophase (P; embryo P1), prometaphase (PM; embryo PM2) and two embryos in metaphase (M1 and M2). For each embryo, data were derived from several segmented areas that were at least 1 µm 2 in size. The total number of holes measured and number of areas per embryo were as follows: prophase, n = 213, nine areas; prometaphase, n = 153, nine areas; M1, n = 58, six areas; and M2, n = 46, five areas. Note that the y axis is discontinuous; blue background highlights the upper segment of the graph (hole area >0.04 µm 2 ). Statistical analyses were done using the Kruskal-Wallis test with correction for multiple comparisons. The adjusted P values for the nonsignificant differences (n.s.) were >0.9999. See for statistical analyses of the lower segment.

Article Snippet: The width of the membrane tubes that form at prometaphase or metaphase between parallel membrane sheets in either the outer–outer junctions or three-way sheet junctions were measured using the Amira 2D scale tool using 3D segmented volumes.

Techniques: Expressing, Imaging, Membrane, Derivative Assay