Immunostaining Phospho-epitopes in Ciliated Organs of Whole Mount Zebrafish Embryos

Sarah C. Rothschild; Ludmila Francescatto; Robert M. Tombes

doi:10.3791/53747

JoVE Journal > Chemistry

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Kimya

免疫染色磷酸化表位整装斑马鱼胚胎纤毛器官

Published: February 19, 2016

doi:

10.3791/53747

Sarah C. Rothschild¹, Ludmila Francescatto², Robert M. Tombes¹

¹Biyoloji Bölümü,Virginia Commonwealth University, ²Center for Human Disease Modeling,Duke University Medical Center

Özet

技术描述于免疫染色在整个斑马鱼胚胎磷酸的表位，然后进行在小至初级纤毛细胞结构双色荧光共焦定位。用于固定和成像技术可以定义位置和特定蛋白质的外观或活化的动力学。

Abstract

细胞迅速增殖，基因的组织特异性表达和信令网络的出现表征所有脊椎动物的早期胚胎发育。即使在单个细胞 – – 动力学和信号的位置，在胚胎发育补充重要的发育基因的鉴定。免疫染色技术描述已被证明以限定小至初级纤毛结构的细胞内和整个动物的信号的动力学。使用激光扫描共聚焦显微镜复合固定，成像和图像处理技术可以在短短36小时内完成。

斑马鱼（ 斑马鱼 ）是谁寻求脊椎动物物种是负担得起的和相关的人类疾病进行研究调查一个理想的有机体。遗传击倒或击倒，必须通过实际的蛋白质产物的损失来确认。蛋白质丢失这样的确认可以使用这里描述的技术来实现。线索到信号通路，也可以通过使用与已经由磷酸化的翻译后修饰的蛋白反应的抗体破译。维护和优化表位的磷酸化状态，因此这一决定的关键，并通过该协议来实现的。

这项研究的发展和第一72小时期间介绍了技术修复的胚胎共定位的各种与在枯否囊泡（KV）纤毛相关的表位，肾脏和内耳。这些技术是简单的，不需要清扫，并可以在一个相对较短的时间内完成。焦投影图像堆栈成一个单一的形象呈现这些数据的有效手段。

Introduction

The techniques described here are the outcome of studies that have sought to define downstream targets of Ca²⁺signals during events that occur during early development, including fertilization, gastrulation, somitogenesis and trunk, eye, brain and organ formation.^1-3 The original discoveries of embryonic Ca²⁺ signaling were dependent on the use of natural and engineered Ca²⁺ indicators, such as aequorin⁴ and fura-2.⁵ Even with current technology, the detection of transient elevations of Ca²⁺ requires cumbersome analytical tools and does not reveal the targets of such Ca²⁺ signals.

This laboratory investigates Ca²⁺ signals that act through the Ca²⁺/calmodulin-dependent (multifunctional) protein kinase known as CaMK-II, an enzyme that is enriched in the central nervous system and originally identified as a regulator of long-term potentiation.⁶ CaMK-II is not brain-specific, is widely expressed and highly conserved throughout the entire lifespan and bodies of species throughout the animal kingdom, including invertebrates.^7,8 CaMK-II has the unique capability of sustaining its own activity even after Ca²⁺ levels have diminished due to its ability to autophosphorylate at Thr²⁸⁷. In this autophosphorylated state, CaMK-II remains active in a Ca²⁺/CaM-independent manner, until dephosphorylated.⁶ Thus, the localization of phosphorylated CaMK-II (Thr²⁸⁷) can identify cells in which natural, relevant Ca²⁺ elevations have occurred.

An antibody against autophosphorylated (P-Thr²⁸⁷) mammalian CaMK-II has been well-characterized and was initially used to localize activated CaMK-II in brain tissue.⁹ Zebrafish (Danio rerio) have seven CaMK-II genes^10,11 whose protein products contain a sequence of MHRQE[pT²⁸⁷]VECLK in this region.^10,11 This sequence is very similar to the phosphopeptide antigen used to create this rabbit polyclonal antibody (MHRQE[pT]VDCLK; Upstate/Millipore) and therefore it was not a complete surprise that this antibody cross-reacted with zebrafish CaMK-II. This laboratory showed that this antibody reacts with zebrafish CaMK-II in proportion to autophosphorylation and Ca²⁺/CaM-independent activity.¹² Additional pan-specific CaMK-II antibodies have also been shown to cross-react with zebrafish CaMK-II.¹³

This antibody has been used to demonstrate that zebrafish CaMK-II is preferentially activated in cells on one side of the zebrafish Kupffer’s Vesicle (KV), the ciliated organ necessary for establishment of left/right asymmetry.¹² This antibody was used to demonstrate that CaMK-II is transiently activated in four adjacent cells on the left side of the KV during the exact same developmental phase that organ positioning is determined.¹² In addition to the Kupffer’s Vesicle (KV), autophosphorylated (P-T²⁸⁷) was also located in specific intracellular sites in other ciliated tissues including the kidney, neuromasts, and inner ear.^12,13 In the zebrafish kidney, P-T²⁸⁷-CaMK-II is enriched along the apical border of ciliated ductal cells and within cloacal cilia where it influences their assembly.¹³ Finally, in the developing inner ear, P-T²⁸⁷-CaMK-II is intensely concentrated at the base of cilia and influences cell differentiation through the Delta-Notch signal pathway.¹⁴ In summary, the detection of activated CaMK-II has pinpointed sites of intracellular Ca²⁺ release and illuminated potential new signaling pathways.

These discoveries were completely dependent on developing a sensitive and accurate method to localize activated (P-T²⁸⁷-autophosphorylated) CaMK-II. The methods to fix and immunostain the zebrafish KV, kidney and inner ear are described. The limitations of this technique are also described. These techniques should be useful to any investigator who seeks to obtain high-resolution images in two fluorescent channels of not just phospho-epitopes, but any epitope, during early vertebrate development.

Protocol

在此协议的斑马鱼程序已经批准的机构动物护理和使用委员会（IACUC）在弗吉尼亚联邦大学。 1.试剂的制备 4％PFA / PBS中。在通风柜权衡，8g仲甲醛（PFA）。同时仍然在通风柜，溶解干燥的PFA在〜80毫升蒸馏H 2ö搅拌并加热至50℃。边搅拌，加3 – 新鲜的1N NaOH 10滴，直到PFA完全溶解，溶液澄清。从火上移开，并加入100 ml 2倍磷酸盐缓冲液（PBS）。带来体积至200毫升…

Representative Results

可视化的磷酸化表位条件最优描述蛋白抗原决定簇在斑马鱼胚胎的免疫组化方法相比，通过原位杂交本地化的mRNAs一直比较稀疏。在定位在斑马鱼胚胎的纤毛细胞蛋白的表位使用的固定剂包括4％PFA / PBS中并登特的固定剂，它是甲醇和DMSO。19定位RNA的由整体原位杂交（WISH）的混合物中，通常?…

Discussion

煤灰/甲醇方法，在这个实验室使用斑马鱼发育期间优化磷酸-T ²⁸⁷ -CaMK-II型表位的免疫定位的主要目的开发的。这种方法的几个纤毛器官，包括斑马鱼^KV，12内耳¹⁴和肾脏^。13特别是在对KV阶段，这种技术是必要的形成过程中成功地本地化的P-钙调蛋白激酶-II该方法的成功可能是由于一个）的自体荧光的最小化，b）该磷钙调蛋白激酶-II型表位的保存和c）的表位的抗体?…

Açıklamalar

The authors have nothing to disclose.

Acknowledgements

这项工作是由美国国家科学基金会资助IOS-0817658的支持。

Materials

1-phenyl-2-thiourea (PTU)	Sigma	P-7629	0.12% Stock solution. Dilute 1:40 in system water
Alexa488 anti-mouse IgG	Life Technologies	A11001	Goat polyclonal, use at 1:500
Alexa488 anti-rabbit IgG	Life Technologies	A11008	Goat polyclonal, use at 1:500
Alexa488 phalloidin	Life Technologies	A12379	Preferentially binds to F-actin
Alexa568 anti-mouse IgG	Life Technologies	A11004	Goat polyclonal, use at 1:500
Alexa568 anti-rabbit IgG	Life Technologies	A11011	Goat polyclonal, use at 1:500
anti-acetylated a-tubulin	Sigma	T7451	Mouse monoclonal, use at 1:500
anti-phospho-T²⁸⁷ CaMK-II	EMD Millipore	06-881	Rabbit polyclonal, use at 1:20
anti-total CaMK-II	BD Biosciences	611292	Mouse monoclonal, use at 1:20
Ethanol	Fisher	S96857	Lab grade, 95% denatured
Forceps	Fine Science Tools	11252-20	Dumont #5
Glass coverslips	VWR	16004-330	#1 thickness
Glass microscope slides	Fisher	12-550-15	Standard glass slides
Methanol	Fisher	A411	Store in freezer
Microcentrifuge tubes	VWR	20170-038	capped tubes, not sterile
Normal goat serum	Life Technologies	16210-064	Aliquot 1ml tubes, store in freezer
Paraformaldehyde	Sigma	P-6148	Reagent grade, crystalline
Phosphate buffered saline (PBS)	Quality Biological	119-069-131	10X stock solution or made in lab
Triton X-100	Sigma	BP-151	10% solution in water, store at room temp
Tween-20	Life Technologies	85113	10% solution in water, store at room temp
Compound microscope	Nikon	E-600	Mount on vibration-free table
C1 Plus two-laser scanning confocal	Nikon	C1 Plus	Run by EZ-C1 program, but upgrades use "Elements"

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Etiketler

Immunostaining Phospho-epitopes Ciliated Organs Whole Mount Zebrafish Embryos Calcium-dependent Signaling Immunolocalization Phosphorylated Proteins Acetylated Tubulin Anti-phospho CaMKII Antibody Fluorescent Secondary Antibody Gelişim Biyolojisi Cell Biology

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Rothschild, S. C., Francescatto, L., Tombes, R. M. Immunostaining Phospho-epitopes in Ciliated Organs of Whole Mount Zebrafish Embryos. J. Vis. Exp. (108), e53747, doi:10.3791/53747 (2016).