Optimized Immunostaining of Embryonic and Early Postnatal Mouse Brain Sections

Kawssar Harb; Michele Bertacchi; Michèle Studer

doi:10.21769/BioProtoc.3868

Optimized Immunostaining of Embryonic and Early Postnatal Mouse Brain Sections

Standard

Optimized Immunostaining of Embryonic and Early Postnatal Mouse Brain Sections. / Harb, Kawssar; Bertacchi, Michele; Studer, Michèle.

In: BIO-PROTOCOL, Vol. 11, No. 1, 05.01.2021, p. e3868.

Research output: SCORING: Contribution to journal › SCORING: Journal article › Research › peer-review

Harvard

Harb, K, Bertacchi, M & Studer, M 2021, 'Optimized Immunostaining of Embryonic and Early Postnatal Mouse Brain Sections', BIO-PROTOCOL, vol. 11, no. 1, pp. e3868. https://doi.org/10.21769/BioProtoc.3868

APA

Harb, K., Bertacchi, M., & Studer, M. (2021). Optimized Immunostaining of Embryonic and Early Postnatal Mouse Brain Sections. BIO-PROTOCOL, 11(1), e3868. https://doi.org/10.21769/BioProtoc.3868

Vancouver

Harb K, Bertacchi M, Studer M. Optimized Immunostaining of Embryonic and Early Postnatal Mouse Brain Sections. BIO-PROTOCOL. 2021 Jan 5;11(1):e3868. https://doi.org/10.21769/BioProtoc.3868

Bibtex

@article{c6b7735b5e1b4408b9dc59514b725812,

title = "Optimized Immunostaining of Embryonic and Early Postnatal Mouse Brain Sections",

abstract = "The mammalian neocortex, the outer layer of the cerebrum and most recently evolved brain region, is characterized by its unique areal and laminar organization. Distinct cortical layers and areas can be identified by the protein expression of graded transcription factors and molecular determinants that define the identity of different projection neurons. Thus, specific detection and visualization of protein expression is crucial for assessing the identity of neocortical neurons and, more broadly, for understanding early and late developmental mechanisms and function of this complex system. Several immunostaining/immunofluorescence methods exist to detect protein expression. Published protocols vary with regard to subtle details, which may impact the final outcome of the immunofluorescence. Here, we provide a detailed protocol, suitable for both thin cryostat sections and thick vibratome sections, which has successfully worked for a wide range of antibodies directed against key molecular players of neocortical development. Ranging from early technical steps of brains collection down to image analysis and statistics, we include every detail concerning sample inclusion and sectioning, slide storage and optimal antibody dilutions aimed at reducing non-specific background. Routinely used in the lab, our background-optimized immunostaining protocol allows efficient detection of area- and layer- specific molecular determinants of distinct neocortical projection neurons. Graphic abstract: Workflow chart for the optimized immunostaining protocol of mouse brain sections. A. A flow chart for different steps of the optimized immunostaining protocol on both thin cryostat and thick vibratome sections. B. Example for immunostaining against Satb2 and Ctip2 on a thin coronal section (20 μm) at the level of the somatosensory cortex. The first column to the left shows the binning system where 6 bins can be overlaid on the image. On the bottom, an example of counting analysis showing the percentage of marker-positive cells normalized to the total number of DAPI or Hoechst-positive cells. C. Example for immunostaining against Satb2 and Ctip2 on a GFP+ thick vibratome section (200 μm). Images are taken at low magnification (10x, left) and high magnification (40x, right). The graph shows a counting of the percentage of Ctip2-positive neurons normalized to the total number of GFP-electroporated neurons on high-magnification images. Images on B and C are modified from Harb et al. (2016).",

author = "Kawssar Harb and Michele Bertacchi and Mich{\`e}le Studer",

note = "Copyright {\textcopyright} The Authors; exclusive licensee Bio-protocol LLC.",

year = "2021",

month = jan,

day = "5",

doi = "10.21769/BioProtoc.3868",

language = "English",

volume = "11",

pages = "e3868",

journal = "BIO-PROTOCOL",

issn = "2331-8325",

publisher = "Sunnyvale, CA",

number = "1",

}

RIS

TY - JOUR

T1 - Optimized Immunostaining of Embryonic and Early Postnatal Mouse Brain Sections

AU - Harb, Kawssar

AU - Bertacchi, Michele

AU - Studer, Michèle

PY - 2021/1/5

Y1 - 2021/1/5

N2 - The mammalian neocortex, the outer layer of the cerebrum and most recently evolved brain region, is characterized by its unique areal and laminar organization. Distinct cortical layers and areas can be identified by the protein expression of graded transcription factors and molecular determinants that define the identity of different projection neurons. Thus, specific detection and visualization of protein expression is crucial for assessing the identity of neocortical neurons and, more broadly, for understanding early and late developmental mechanisms and function of this complex system. Several immunostaining/immunofluorescence methods exist to detect protein expression. Published protocols vary with regard to subtle details, which may impact the final outcome of the immunofluorescence. Here, we provide a detailed protocol, suitable for both thin cryostat sections and thick vibratome sections, which has successfully worked for a wide range of antibodies directed against key molecular players of neocortical development. Ranging from early technical steps of brains collection down to image analysis and statistics, we include every detail concerning sample inclusion and sectioning, slide storage and optimal antibody dilutions aimed at reducing non-specific background. Routinely used in the lab, our background-optimized immunostaining protocol allows efficient detection of area- and layer- specific molecular determinants of distinct neocortical projection neurons. Graphic abstract: Workflow chart for the optimized immunostaining protocol of mouse brain sections. A. A flow chart for different steps of the optimized immunostaining protocol on both thin cryostat and thick vibratome sections. B. Example for immunostaining against Satb2 and Ctip2 on a thin coronal section (20 μm) at the level of the somatosensory cortex. The first column to the left shows the binning system where 6 bins can be overlaid on the image. On the bottom, an example of counting analysis showing the percentage of marker-positive cells normalized to the total number of DAPI or Hoechst-positive cells. C. Example for immunostaining against Satb2 and Ctip2 on a GFP+ thick vibratome section (200 μm). Images are taken at low magnification (10x, left) and high magnification (40x, right). The graph shows a counting of the percentage of Ctip2-positive neurons normalized to the total number of GFP-electroporated neurons on high-magnification images. Images on B and C are modified from Harb et al. (2016).

AB - The mammalian neocortex, the outer layer of the cerebrum and most recently evolved brain region, is characterized by its unique areal and laminar organization. Distinct cortical layers and areas can be identified by the protein expression of graded transcription factors and molecular determinants that define the identity of different projection neurons. Thus, specific detection and visualization of protein expression is crucial for assessing the identity of neocortical neurons and, more broadly, for understanding early and late developmental mechanisms and function of this complex system. Several immunostaining/immunofluorescence methods exist to detect protein expression. Published protocols vary with regard to subtle details, which may impact the final outcome of the immunofluorescence. Here, we provide a detailed protocol, suitable for both thin cryostat sections and thick vibratome sections, which has successfully worked for a wide range of antibodies directed against key molecular players of neocortical development. Ranging from early technical steps of brains collection down to image analysis and statistics, we include every detail concerning sample inclusion and sectioning, slide storage and optimal antibody dilutions aimed at reducing non-specific background. Routinely used in the lab, our background-optimized immunostaining protocol allows efficient detection of area- and layer- specific molecular determinants of distinct neocortical projection neurons. Graphic abstract: Workflow chart for the optimized immunostaining protocol of mouse brain sections. A. A flow chart for different steps of the optimized immunostaining protocol on both thin cryostat and thick vibratome sections. B. Example for immunostaining against Satb2 and Ctip2 on a thin coronal section (20 μm) at the level of the somatosensory cortex. The first column to the left shows the binning system where 6 bins can be overlaid on the image. On the bottom, an example of counting analysis showing the percentage of marker-positive cells normalized to the total number of DAPI or Hoechst-positive cells. C. Example for immunostaining against Satb2 and Ctip2 on a GFP+ thick vibratome section (200 μm). Images are taken at low magnification (10x, left) and high magnification (40x, right). The graph shows a counting of the percentage of Ctip2-positive neurons normalized to the total number of GFP-electroporated neurons on high-magnification images. Images on B and C are modified from Harb et al. (2016).

U2 - 10.21769/BioProtoc.3868

DO - 10.21769/BioProtoc.3868

M3 - SCORING: Journal article

C2 - 33732758

VL - 11

SP - e3868

JO - BIO-PROTOCOL

JF - BIO-PROTOCOL

SN - 2331-8325

IS - 1

ER -