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Thermo Fisher Scientific • 5791 Van Allen Way • Carlsbad, CA 92008 • www.thermofisher.com
Click Colorimetric EdU Proliferation and TUNEL: Click Chemistry for
Bright Field Microscopy
Scott T. Clarke1, Carmen Finnessy1, Fernada M. Bosada2, Ben Armstrong2, and Michael O’Grady1
1Molecular Probes Labeling and Detection, Thermo Fisher Scientific, Eugene, Oregon, USA; 2Institute of Molecular Biology, University of Oregon, Eugene, Oregon, USA
EdU/BrdU double labeling in rat epithelium
Figure 3: EdU labeling combined with Movat’s Pentachrome stain shows
compatibility of DAB with multiple color pentachrome staining. Longitudinal section
through the crypts shows proliferating cell locally abundant near the base of the crypts and diminishing
with distance. Proliferating cells (brown) signal is visible against Movat’s Pentachrome staining consisting
of Verhoeff-Van Gieson’s staining of elastin (black) and nuclei (purplish gray), alcoholic saffron staining of
collagen (yellow), Alcian Blue staining of mucins marking the goblet cells (blue), and Crocein Scarlet -
Acid Fuchsin staining of muscle and red blood cells (red). Imaged with 20X objective
ABSTRACT AND INTRODUCTION
We present the conversion of click chemistry EdU and TUNEL fluorescence
assay to colorimetric detection of proliferation and apoptosis for use with bright
field microscopy. Advantages of having a click colorimetric signal are retaining
the work flow of click chemistry labeling while allowing for compatibility with
standard H&E staining and protocols.
While antibody based BrdU and BrdUTP used for proliferation and TUNEL assays
is detected with a colorimetric reagent, EdU and EdUTP, which uses click
chemistry for detection, has not previously been reported.
Although fluorescence based detection is a standard practice which allows for
multiplexing with other antibody based markers, there are occasions when
colorimetric labeling is needed to avoid tissue auto-fluorescence, or to be
compatible with standard histological stains for morphological and contextual
information.
Both click chemistry EdU and TUNEL staining are compatible with hematological
stains and show contextual environment. Additionally, two color proliferation
using EdU/BrdU dual pulse labeled tissue using colorimetric substrates for
horseradish peroxidase and alkaline phosphatase.
MATERIALS AND METHODS
For Zebrafish caudal fin regeneration 50 nmoles EdU i.p. was pulsed 48 hours
after amputation for 5 hours prior to sacrifice. Caudal fin tissue was fixed in 10%
formalin overnight, washed then decalcified with EDTA for 4 days then
dehydrated prior to paraffin embedding and 7 mm sectioning.
For mouse heart tissue EdU/BrdU double labeling was performed using 50 mg/g
i.p. injection of BrdU once daily for 6 days followed by a single injection of 50 mg/g
EdU 24 hours prior to sacrifice. Cardiac tissue was prepared in 10% formalin
overnight and stored in 70% ethanol prior to paraffin embedding and 5 mm
sectioning.
For rat uterine EdU/BrdU double labeling was performed by hormonally inducing
proliferation in adolescent female rats by administering 200 mg estradiol-17b in
silastic tubing over the course of 7 days prior to 160 mg/g of either BrdU or EdU
injection i.p. After either 3 or 7 days the other thymidine analog was administered
2 hours prior to sacrifice. Uterine and intestinal tissue were prepared in 10%
formalin overnight and stored in 70% ethanol prior to paraffin embedding and 8
mm sectioning.
All experimental treatments followed IACUC and NIH guidelines for care and use
of the animals.
For detection Click-iT™ EdU Colorimetric IHC Detection kit and Click-iT™ TUNEL
Colorimetric IHC Detection kit were performed following manufacture’s
instructions (Thermo Fisher Scientific). Briefly, the tissue was de-paraffinization in
xylene and hydrated in graded alcohol baths, peroxidase quenched and
enzymatically digested prior to click labeling. BrdU detection required additional
treatment with HCl treatment for DNA revelation. Antibodies for BrdU (mouse
clone MoBU-1), and (goat anti-mouse alkaline phosphatase were used on rat
tissue. Antibodies for BrdU (rat clone BU1/75) and donkey anti-rat alkaline
phosphatase (Jackson ImmunoResearch) were used on mouse tissue.
Chromogens used for colorimetric detection include Russell-Movats Pentachrome
(American MasterTech) following EdU detection with DAB. For EdU/BrdU double
labeling Vector™ Blue was combined with Vector™ NovaRed™ (Vector
Laboratories)
All images acquired with the color camera on the EVOS™ FL Auto Cell Imaging
System.
All reagents were obtained from Thermo Fisher Scientific unless otherwise noted.
ACKNOWLEDGEMENTS
We gratefully acknowledge Rajkumar Lakshmanaswamy and Arunkumar Arumugam from Texas Tech
University Health Sciences Center for the preparation of the dual pulse labeled rat tissue.
Figure 2: EdU labeling with Click-iT EdU Colorimetric IHC kit. 8 mm FFPE section of rat
intestine was labeled with DAB showing proliferating (brown nuclei) and counterstained with Meyer’s
hematoxylin showing non-proliferating cells (blue nuclei). Image acquired using 20X objective.
200 ms
Time 0
Proliferation (EdU labeled) with Movat’s Pentachrome
staining in rat intestine
Figure 4: EdU/BrdU double labeling of proliferating cells of rat vaginal epithelium.
EdU (red-brown) and BrdU (blue). EdU pulsed first followed by BrdU 3 days later shows distribution of
EdU labeled cells within the vaginal epithelial layer while newly formed BrdU cells are seen adjacent to
the basement membrane. Imaged wet mounted in PBS with 20X objective
Proliferation (EdU) with hematoxylin staining
Proliferating cells in mouse heart valve labeled
with EdU and Movat’s Pentachrome stain
Figure 5: EdU labeling with Movat’s Pentachrome stain highlights proliferating
cell population in Zebrafish caudal fin regeneration model. Dashed line showing the
approximate location of amputation and subsequent regrowth after 48 hrs. Proliferating cells (brown)
forming both in the regenerated fin and pre-existing tissue. Existing bone and cartilage (red and yellow)
stained with Crocein Scarlet - Acid Fuchsin and alcoholic saffron. Mucins (blue) stained with Alcian
Blue. Non proliferating cells stained gray. Multiple image stitched using EVOS software (20X objective)
For Research Use Only. Not for use in diagnostic procedures
© 2016 Thermo Fisher Scientific Inc. All rights reserved.
All trademarks are the property of Thermo Fisher Scientific and
its subsidiaries unless otherwise specified.
Figure 6: EdU labeling with Movat’s Pentachrome stain through transverse
sections of mouse cardiac tissue. Enlarged magnification of DPN0 stage of mouse section # 6
showing the three leaflets of the heart valve with proliferating EdU labeled cells (dark brown) and non-
proliferating cells (gray) surrounded by artery wall staining positive for elastin (black), and collagen
(yellow), along with muscle (dark red) and red blood cells (bright red). Imaged with 20X objective on
EVOS FL Auto Cell Imaging System.
EdU with Movat’s in Zebrafish caudal fin tissue
a
Click-iT labeling
biotin azide
Cu (I) biotin
EdU or EdUTP
labeled
DNA
DABSA-HRP
Click chemistry TUNEL staining in mouse thymus
Figure 1: Apoptosis labeling with Click-iT TUNEL colorimetric IHC kit. 1A: 8 mm
FFPE section of mouse thymus was labeled with DAB for TUNEL-positive cells (brown nuclei) and
counterstained with Eosin Y (pink), and Methyl Green (green), dehydrated, and hard mounted in
Cytoseal™ 60. 1B: mouse intestine showing apoptosis in TUNEL positive cells stained with DAB. 1C:
TUNEL staining (brown) in mouse brain tissue combined with Luxol Fast Blue which stains myelin fibers
(blue/turquoise), nuclei (purple/violet) and Nissl substance (purple/violet). All images were acquired using
a 20X objective on an EVOS FL Auto Imaging Station equipped with a color camera.
EdU and TUNEL colorimetric labeling strategy

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Click Colorimetric EdU Proliferation and TUNEL: Click Chemistry for Bright Field Microscopy

  • 1. Thermo Fisher Scientific • 5791 Van Allen Way • Carlsbad, CA 92008 • www.thermofisher.com Click Colorimetric EdU Proliferation and TUNEL: Click Chemistry for Bright Field Microscopy Scott T. Clarke1, Carmen Finnessy1, Fernada M. Bosada2, Ben Armstrong2, and Michael O’Grady1 1Molecular Probes Labeling and Detection, Thermo Fisher Scientific, Eugene, Oregon, USA; 2Institute of Molecular Biology, University of Oregon, Eugene, Oregon, USA EdU/BrdU double labeling in rat epithelium Figure 3: EdU labeling combined with Movat’s Pentachrome stain shows compatibility of DAB with multiple color pentachrome staining. Longitudinal section through the crypts shows proliferating cell locally abundant near the base of the crypts and diminishing with distance. Proliferating cells (brown) signal is visible against Movat’s Pentachrome staining consisting of Verhoeff-Van Gieson’s staining of elastin (black) and nuclei (purplish gray), alcoholic saffron staining of collagen (yellow), Alcian Blue staining of mucins marking the goblet cells (blue), and Crocein Scarlet - Acid Fuchsin staining of muscle and red blood cells (red). Imaged with 20X objective ABSTRACT AND INTRODUCTION We present the conversion of click chemistry EdU and TUNEL fluorescence assay to colorimetric detection of proliferation and apoptosis for use with bright field microscopy. Advantages of having a click colorimetric signal are retaining the work flow of click chemistry labeling while allowing for compatibility with standard H&E staining and protocols. While antibody based BrdU and BrdUTP used for proliferation and TUNEL assays is detected with a colorimetric reagent, EdU and EdUTP, which uses click chemistry for detection, has not previously been reported. Although fluorescence based detection is a standard practice which allows for multiplexing with other antibody based markers, there are occasions when colorimetric labeling is needed to avoid tissue auto-fluorescence, or to be compatible with standard histological stains for morphological and contextual information. Both click chemistry EdU and TUNEL staining are compatible with hematological stains and show contextual environment. Additionally, two color proliferation using EdU/BrdU dual pulse labeled tissue using colorimetric substrates for horseradish peroxidase and alkaline phosphatase. MATERIALS AND METHODS For Zebrafish caudal fin regeneration 50 nmoles EdU i.p. was pulsed 48 hours after amputation for 5 hours prior to sacrifice. Caudal fin tissue was fixed in 10% formalin overnight, washed then decalcified with EDTA for 4 days then dehydrated prior to paraffin embedding and 7 mm sectioning. For mouse heart tissue EdU/BrdU double labeling was performed using 50 mg/g i.p. injection of BrdU once daily for 6 days followed by a single injection of 50 mg/g EdU 24 hours prior to sacrifice. Cardiac tissue was prepared in 10% formalin overnight and stored in 70% ethanol prior to paraffin embedding and 5 mm sectioning. For rat uterine EdU/BrdU double labeling was performed by hormonally inducing proliferation in adolescent female rats by administering 200 mg estradiol-17b in silastic tubing over the course of 7 days prior to 160 mg/g of either BrdU or EdU injection i.p. After either 3 or 7 days the other thymidine analog was administered 2 hours prior to sacrifice. Uterine and intestinal tissue were prepared in 10% formalin overnight and stored in 70% ethanol prior to paraffin embedding and 8 mm sectioning. All experimental treatments followed IACUC and NIH guidelines for care and use of the animals. For detection Click-iT™ EdU Colorimetric IHC Detection kit and Click-iT™ TUNEL Colorimetric IHC Detection kit were performed following manufacture’s instructions (Thermo Fisher Scientific). Briefly, the tissue was de-paraffinization in xylene and hydrated in graded alcohol baths, peroxidase quenched and enzymatically digested prior to click labeling. BrdU detection required additional treatment with HCl treatment for DNA revelation. Antibodies for BrdU (mouse clone MoBU-1), and (goat anti-mouse alkaline phosphatase were used on rat tissue. Antibodies for BrdU (rat clone BU1/75) and donkey anti-rat alkaline phosphatase (Jackson ImmunoResearch) were used on mouse tissue. Chromogens used for colorimetric detection include Russell-Movats Pentachrome (American MasterTech) following EdU detection with DAB. For EdU/BrdU double labeling Vector™ Blue was combined with Vector™ NovaRed™ (Vector Laboratories) All images acquired with the color camera on the EVOS™ FL Auto Cell Imaging System. All reagents were obtained from Thermo Fisher Scientific unless otherwise noted. ACKNOWLEDGEMENTS We gratefully acknowledge Rajkumar Lakshmanaswamy and Arunkumar Arumugam from Texas Tech University Health Sciences Center for the preparation of the dual pulse labeled rat tissue. Figure 2: EdU labeling with Click-iT EdU Colorimetric IHC kit. 8 mm FFPE section of rat intestine was labeled with DAB showing proliferating (brown nuclei) and counterstained with Meyer’s hematoxylin showing non-proliferating cells (blue nuclei). Image acquired using 20X objective. 200 ms Time 0 Proliferation (EdU labeled) with Movat’s Pentachrome staining in rat intestine Figure 4: EdU/BrdU double labeling of proliferating cells of rat vaginal epithelium. EdU (red-brown) and BrdU (blue). EdU pulsed first followed by BrdU 3 days later shows distribution of EdU labeled cells within the vaginal epithelial layer while newly formed BrdU cells are seen adjacent to the basement membrane. Imaged wet mounted in PBS with 20X objective Proliferation (EdU) with hematoxylin staining Proliferating cells in mouse heart valve labeled with EdU and Movat’s Pentachrome stain Figure 5: EdU labeling with Movat’s Pentachrome stain highlights proliferating cell population in Zebrafish caudal fin regeneration model. Dashed line showing the approximate location of amputation and subsequent regrowth after 48 hrs. Proliferating cells (brown) forming both in the regenerated fin and pre-existing tissue. Existing bone and cartilage (red and yellow) stained with Crocein Scarlet - Acid Fuchsin and alcoholic saffron. Mucins (blue) stained with Alcian Blue. Non proliferating cells stained gray. Multiple image stitched using EVOS software (20X objective) For Research Use Only. Not for use in diagnostic procedures © 2016 Thermo Fisher Scientific Inc. All rights reserved. All trademarks are the property of Thermo Fisher Scientific and its subsidiaries unless otherwise specified. Figure 6: EdU labeling with Movat’s Pentachrome stain through transverse sections of mouse cardiac tissue. Enlarged magnification of DPN0 stage of mouse section # 6 showing the three leaflets of the heart valve with proliferating EdU labeled cells (dark brown) and non- proliferating cells (gray) surrounded by artery wall staining positive for elastin (black), and collagen (yellow), along with muscle (dark red) and red blood cells (bright red). Imaged with 20X objective on EVOS FL Auto Cell Imaging System. EdU with Movat’s in Zebrafish caudal fin tissue a Click-iT labeling biotin azide Cu (I) biotin EdU or EdUTP labeled DNA DABSA-HRP Click chemistry TUNEL staining in mouse thymus Figure 1: Apoptosis labeling with Click-iT TUNEL colorimetric IHC kit. 1A: 8 mm FFPE section of mouse thymus was labeled with DAB for TUNEL-positive cells (brown nuclei) and counterstained with Eosin Y (pink), and Methyl Green (green), dehydrated, and hard mounted in Cytoseal™ 60. 1B: mouse intestine showing apoptosis in TUNEL positive cells stained with DAB. 1C: TUNEL staining (brown) in mouse brain tissue combined with Luxol Fast Blue which stains myelin fibers (blue/turquoise), nuclei (purple/violet) and Nissl substance (purple/violet). All images were acquired using a 20X objective on an EVOS FL Auto Imaging Station equipped with a color camera. EdU and TUNEL colorimetric labeling strategy