Dissection and Explant Culture of Murine Allantois for the <em>In Vitro</em> Analysis of Allantoic Attachment

Kerstin Hadamek; Angelika Keller; Antje Gohla

doi:10.3791/56712

JoVE Journal > Medicine

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Medicine

郭清と尿の添付ファイルのIn Vitro解析マウス尿膜の培養

Published: January 13, 2018

doi:

10.3791/56712

Kerstin Hadamek², Angelika Keller², Antje Gohla²

¹Institute of Pharmacology and Toxicology,University of Würzburg, ²Rudolf Virchow Center for Experimental Biomedicine,University of Würzburg

Summary

モデル漿添付ファイル、胎盤形成の最初のステップの in vitroアッセイについて述べる。プロトコルは、固定化 α4β1 インテグリンのマウス allantoides の郭清と植の文化を示しています。尿膜の添付ファイルは、あらかじめ決められた時点で病理組織学的に評価されます。

Abstract

胎盤は、成長と哺乳動物の胎児の開発のために不可欠です。このため、多数の遺伝子変異と胎盤の開発または機能を妨げる可能性が高いのも環境の侮辱が、マウスとヒトの妊娠初期の損失にあります。それにもかかわらず、画面の胎盤形成に対する潜在的な影響に簡単な生体外の試金が不足しています。ここでは、モデリングにおける胎盤絨毛膜に尿膜壁添付ファイルから成っている最初の重要なステップに焦点を当てます。Chorio 擬態の基板となる固定化 α4β1 インテグリンの尿外植片の添付ファイルを迅速に評価する方法について述べる。この体外アプローチにより、添付ファイルと異なる連続した時点で複数の尿膜外植体の挙動を拡散の定性的な評価です。プロトコルは、ターゲットを絞ったマウス突然変異、薬、または妊娠合併症や尿膜添付ファイル前のヴィヴォの胎児の損失にリンクされているさまざまな環境要因の効果を調べるために使えます。

Introduction

胎盤が子宮環境の胚の成長と開発のために不可欠です。それは内分泌と免疫器官としての酸素代謝物、胎児と母体の循環とも機能間の栄養交換のためのインターフェイスを構成します。胎盤発育を損なう内因性または外因性の侮辱は、子宮内胎児発育遅延、胎児の損失、または妊娠合併症、マウスと人間¹の両方につながることができます。対象となるマウスを異常な胎盤の生理を引き起こす突然変異の数が 219 遺伝子多型のマウスのゲノム情報学 (MGI) ウェブサイトに現在表示されている²を増やす続けます (http://www.informatics.jax.org/vocab/ mp_ontology/MP:0010038)、これらの表現型の多くはよく機械論的視点から理解されていません。に加えて遺伝子変異、小分子薬、モノクローナル抗体、毒素、病原体、余分な代謝物や様々な環境要因や影響を与える胎盤開発関数³^,⁴^,⁵^,⁶^,⁷します。まだ、簡単な生体外モデル胎盤の開発で重要な手順が不足している試金。

(臍帯発達前駆体) 尿膜が絨毛膜⁸に向かって育つ芽として胚の後部の端から現れるとき、初期の経産婦でマウス胎盤の発育が開始されます。尿の芽の外側の層の Chorioadhesive セルは、添付ファイルおよび絨毛膜 (漿「融合」) の表面に尿膜の広がりを仲介します。絨毛膜はその後に尿膜壁血管成長迷路、栄養素と酸素が密接に並置母体血と胎児血管^{9 間交換される胎盤内層を形成する絨毛に折る} ^,¹⁰。

絨毛膜へ尿の付着迷宮形成の初期および重要なステップであり、このプロセスの欠陥は midgestation¹胚性致死性の最も一般的な原因のうち。マウス突然変異体の数が、漿添付ファイル¹⁰が発生するが失敗し、MGI データベース現在異常な漿融合 (http:// によって特徴付けられる 108 マウスの突然変異体の一覧を記載されてwww.informatics.jax.org/vocab/mp_ontology/MP:0002824)、血管細胞接着分子 1 (VCAM 1、尿中胚葉に発現) と (は絨毛の中皮に表される α4β1 インテグリンの細胞間相互作用初期胚胚体外胚葉由来) 漿添付ファイルと融合¹¹^,¹²^,¹³のため不可欠であることが表示されます。(E) 7.5 日約 VCAM 1 が尿の茎の遠位 3 分の 2 以内単位があることを示している全体マウント野生型胚の免疫組織化学的染色¹³ (1-4 体節期)、およびその発現状態のまま高漿の添付ファイルと – 融合¹¹^,¹²。絨毛膜尿愛着の障害は、通常、子宮の芽の組織学的解析による検出します。ただし、尿膜サイズはの間と同じ発達段階¹⁴リットル内でも高い生理学的変数であり、尿は、物理的な接触をするのに十分な大きさに達したときに絨毛膜にのみ添付できます。この自然の変動を反映して、漿添付が行われる間のいつか〜 E 8.0 と 9.0 E子宮内、および組織によって、このプロセスの統計的信頼性の高い評価は大きい数の解析に依存したがって淘汰適切な発達段階で十分な検体を採取します。

ここでは、尿の添付ファイル子宮 ex少ない尿膜のサイズに依存している評価方法について述べる。妊娠マウスの子宮からマウス胚とその allantoides の郭清を紹介〜 8 日のポストの coitum 定め(dpc; dpc 0.5 が膣にプラグインの検出を示す)、固定化 α4β1 の外植体尿膜の後続の文化とインテグリンです。このメソッドは、添付ファイルおよび複数並列で、異なる連続した時点で尿膜外植体の挙動を広がりの急速な機能評価できます。プロトコルを使用することがあります尿膜添付ファイル前のヴィヴォに及ぼすターゲット変異、薬、または様々な環境要因の画面に。

Protocol

マウス繁殖は Regierung Unterfranken によって承認された、すべてのドイツ語、欧州連合の法律、実験動物の管理と使用に関する規制に従い、すべての解析を行った。 1. コーティングのマイクロタイタープレート α4β1 インテグリンとEx 子宮尿膜培養 200 μ g/mL 滅菌リン酸緩衝生理食塩水 (PBS) で凍結乾燥させたマウス α4β1 インテグリンを再構成します。予め温め…

Representative Results

このプロトコルを特定しマウス allantoides前のヴィヴォ、外植体について述べるし、体内漿融合中 α4β1 インテグリンに尿膜添付ファイル、重要なプロセスの定性的な評価の詳細。図 1 a-Hに示す代表的な結果は、妊娠子宮から始まって尿膜分離の連続した手順を示します。脂肪組織と血管 (図 1…

Discussion

プロの接着細胞外マトリックス分子フィブロネクチンなどの豊富な源である血清の存在下で尿膜外植体は容易に様々なプラスチックやガラス、フィルター表面⁹^,¹⁶にアタッチされます。したがって、実行される分析の目的は、遺伝子組み換えの効果を具体的に検討する場合、尿膜の添付ファイルに他の処理固定化 α4β1 は、非特異的結合部位 (例?…

Disclosures

The authors have nothing to disclose.

Acknowledgements

この作品は、(社) にドイツ研究振興協会 SFB688 によって支えられました。

Materials

C57BL/6J wildtype mice The Jackson Laboratory Stock No: 000664

70 % (v/v) Ethanol VWR International 930031006

Standard pattern forceps Fine Science Tools 11000-12 Forceps used to open the abdominal cavity.

Micro dissecting forceps Fine Science Tools 11254-20 Dumont # 5 medical biology forcepts with fine, sharp tip.

Fine scissors Fine Science Tools 14094-11 Straight blades.

Spring scissors Fine Science Tools 15012-12 Noyes spring scissors with 14 mm blades for the dissection of uterus buds.

Microspoon Carl Roth AT18.1 5 mm Spoon diameter.

Microtiter plates ibidi 81501 We use uncoated, sterile angiogenesis slides (internal volume 50 µL) with a hydrophobic surface that is not tissue-culture treated to reduce non-a4b1-mediated binding to plastic.

10 cm dish Nunc 150350 Sterile tissue culture dishes.

3.5 cm dish Nunc 150288 Sterile tissue culture dishes.

Large orifice pipette tips Biozym VT0140X Low binding pipette tips, 200 µL.

a4b1 integrin R&D Systems 6054-A4 Murine a4b1 integrin recombinantly expressed and purified from a Chinese hamster ovary cell line.

Dulbecco's Phosphate Buffered Saline (PBS) Sigma Aldrich D8537 Without Ca²⁺ and Mg²⁺.

Dulbecco’s Modified Eagle Medium (DMEM) PAN Biotech P04-03600 The formulation contains 4.5 g/L glucose, 110 mg/L sodium pyruvate and 3.7 g/L NaHCO₃ but no L-glutamine, which is added separately.

Penicillin/Streptomycin Gibco (ThermoFisher Scientific) 15140-122 100 x (10,000 U/mL Penicillin and 10,000 µg/mL streptomycin) stock solution. Prepare and store aliquots at -20 °C to avoid freeze/thaw.

L-Glutamine PAN Biotech P04-80100 100 x (200 mM) Stock solution. Prepare and store aliquots at -20 °C to avoid freeze/thaw.

Fetal bovine serum Biochrom S 0115 We use heat-inactivated FBS (heated to 56 °C for 30 min with mixing to inactivate complement).

Bovine serum albumin (BSA) Sigma Aldrich A7030 We use protease- and fatty acid-free albumin. Prepare a 0.1 % (w/v) solution in DMEM. Sterile filter the solution through a disposable cell culture filter with a 0.22 µm pore size and low protein-binding membrane, and store aliquots at -20 °C.

para-Formaldehyde Carl Roth 0335.2 To make a formaldehyde solution in PBS, weigh para-formaldehyde powder in a ventilated hood, and add it to PBS preheated to ca. 60 °C in a beaker on a stir plate. Add 1 N NaOH dropwise until solution clears. Let solution cool to room temperature, and filter through 0.22 mm filter syringe. Adjust pH with diluted HCl to ca. 6.9, and adjust to final volume with PBS. We aliquot and freeze the solution, but it can also be stored at 4 °C for approximately four weeks.

Triton X-100 Sigma Aldrich X100 Use wide-orifice pipette tips to handle undiluted Triton X-100.

Normal goat serum Sigma Aldrich G9023 To block non-specific binding of antibodies in immunofluorescence analyses.

a-CD31 Antibodies BD Biosciences 550274 Purified rat anti-mouse monoclonal antibodies, clone MEC 13.3.

Secondary goat anti-rat antibodies Thermo Fisher A-11006 Goat anti-rat IgG (heavy and light chains), cross-adsorbed, fluorescently labeled with Alexa Fluor 488. Other fluorescent labels are also possible.

Mowiol 4-88 Sigma Aldrich 81381 Mounting medium for cytochemistry. MW ~31,000

Labovert Leitz Labovert Inverted phase contrast microscope equipped with a 4 x and 10 x objective for somite pair counting. Other phase contrast microscopes (such as those that are routinely used in tissue culture) are also suitable.

M80 Leica Microsystems M80 Stereomicroscope with 8 : 1 zoom range (yielding a magnification between 7.5 x and 60 x) for embryo and allantois dissection.

DM4000B Leica Microsystems DM4000B Microscope system for histology with LED illumination. We use HCX PL FLUOTAR 5 x/0.15 and HC PL FLUOTAR 10 x/0.30 objectives. Other microscopes equipped phase contrast and fluorescence optics can be used to score allantois attachment.

Digital camera JVC KY-F75U 3-CCD digital capture camera attached to the DM4000B LED microscope. We use Diskus software (Hilgers) to operate both the microscope and the camera.

Confocal microscope Leica Microsystems SP5 Confocal microscope for higher-resolution imaging of endothelia in the vascular plexus of allantois explants. Immunofluorescence images were taken with a 40 x objective.

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Tags

Murine Allantois Allantoic Attachment Placenta Formation Embryo Development In Vitro Analysis Alpha 4/beta 1 Integrin Explant Culture Dissection Uterus Mouse Embryo

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Hadamek, K., Keller, A., Gohla, A. Dissection and Explant Culture of Murine Allantois for the In Vitro Analysis of Allantoic Attachment. J. Vis. Exp. (131), e56712, doi:10.3791/56712 (2018).

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C57BL/6J wildtype mice	The Jackson Laboratory	Stock No: 000664
70 % (v/v) Ethanol	VWR International	930031006
Standard pattern forceps	Fine Science Tools	11000-12	Forceps used to open the abdominal cavity.
Micro dissecting forceps	Fine Science Tools	11254-20	Dumont # 5 medical biology forcepts with fine, sharp tip.
Fine scissors	Fine Science Tools	14094-11	Straight blades.
Spring scissors	Fine Science Tools	15012-12	Noyes spring scissors with 14 mm blades for the dissection of uterus buds.
Microspoon	Carl Roth	AT18.1	5 mm Spoon diameter.
Microtiter plates	ibidi	81501	We use uncoated, sterile angiogenesis slides (internal volume 50 µL) with a hydrophobic surface that is not tissue-culture treated to reduce non-a4b1-mediated binding to plastic.
10 cm dish	Nunc	150350	Sterile tissue culture dishes.
3.5 cm dish	Nunc	150288	Sterile tissue culture dishes.
Large orifice pipette tips	Biozym	VT0140X	Low binding pipette tips, 200 µL.
a4b1 integrin	R&D Systems	6054-A4	Murine a4b1 integrin recombinantly expressed and purified from a Chinese hamster ovary cell line.
Dulbecco's Phosphate Buffered Saline (PBS)	Sigma Aldrich	D8537	Without Ca²⁺ and Mg²⁺.
Dulbecco’s Modified Eagle Medium (DMEM)	PAN Biotech	P04-03600	The formulation contains 4.5 g/L glucose, 110 mg/L sodium pyruvate and 3.7 g/L NaHCO₃ but no L-glutamine, which is added separately.
Penicillin/Streptomycin	Gibco (ThermoFisher Scientific)	15140-122	100 x (10,000 U/mL Penicillin and 10,000 µg/mL streptomycin) stock solution. Prepare and store aliquots at -20 °C to avoid freeze/thaw.
L-Glutamine	PAN Biotech	P04-80100	100 x (200 mM) Stock solution. Prepare and store aliquots at -20 °C to avoid freeze/thaw.
Fetal bovine serum	Biochrom	S 0115	We use heat-inactivated FBS (heated to 56 °C for 30 min with mixing to inactivate complement).
Bovine serum albumin (BSA)	Sigma Aldrich	A7030	We use protease- and fatty acid-free albumin. Prepare a 0.1 % (w/v) solution in DMEM. Sterile filter the solution through a disposable cell culture filter with a 0.22 µm pore size and low protein-binding membrane, and store aliquots at -20 °C.
para-Formaldehyde	Carl Roth	0335.2	To make a formaldehyde solution in PBS, weigh para-formaldehyde powder in a ventilated hood, and add it to PBS preheated to ca. 60 °C in a beaker on a stir plate. Add 1 N NaOH dropwise until solution clears. Let solution cool to room temperature, and filter through 0.22 mm filter syringe. Adjust pH with diluted HCl to ca. 6.9, and adjust to final volume with PBS. We aliquot and freeze the solution, but it can also be stored at 4 °C for approximately four weeks.
Triton X-100	Sigma Aldrich	X100	Use wide-orifice pipette tips to handle undiluted Triton X-100.
Normal goat serum	Sigma Aldrich	G9023	To block non-specific binding of antibodies in immunofluorescence analyses.
a-CD31 Antibodies	BD Biosciences	550274	Purified rat anti-mouse monoclonal antibodies, clone MEC 13.3.
Secondary goat anti-rat antibodies	Thermo Fisher	A-11006	Goat anti-rat IgG (heavy and light chains), cross-adsorbed, fluorescently labeled with Alexa Fluor 488. Other fluorescent labels are also possible.
Mowiol 4-88	Sigma Aldrich	81381	Mounting medium for cytochemistry. MW ~31,000
Labovert	Leitz	Labovert	Inverted phase contrast microscope equipped with a 4 x and 10 x objective for somite pair counting. Other phase contrast microscopes (such as those that are routinely used in tissue culture) are also suitable.
M80	Leica Microsystems	M80	Stereomicroscope with 8 : 1 zoom range (yielding a magnification between 7.5 x and 60 x) for embryo and allantois dissection.
DM4000B	Leica Microsystems	DM4000B	Microscope system for histology with LED illumination. We use HCX PL FLUOTAR 5 x/0.15 and HC PL FLUOTAR 10 x/0.30 objectives. Other microscopes equipped phase contrast and fluorescence optics can be used to score allantois attachment.
Digital camera	JVC	KY-F75U	3-CCD digital capture camera attached to the DM4000B LED microscope. We use Diskus software (Hilgers) to operate both the microscope and the camera.
Confocal microscope	Leica Microsystems	SP5	Confocal microscope for higher-resolution imaging of endothelia in the vascular plexus of allantois explants. Immunofluorescence images were taken with a 40 x objective.