我们要感谢 Jennifer A. Zallen 博士提供 Sqh-GFP 果蝇 品系并为该技术的初始开发提供支持，并感谢 Francois Schweisguth 博士提供 Notch-GFP 果蝇 品系。这项工作得到了中国国家自然科学基金（32270809）对H.H.Yu的资助，南方科技大学生命科学学院的慷慨资助和人员支持，以及深圳市科学技术创新委员会/JCYJ20200109140201722对Y. Yan的资助。

实验是按照南方科技大学生命科学学院的指导和批准进行的。使用的生物体是黑腹果蝇，基因型是Notch-Knockin-GFP（X染色体）和Sqh-sqh-GFP（染色体II），分别由Francois Schweisguth博士（巴斯德研究所）和Jennifer Zallen博士（斯隆凯特琳研究所）的实验室慷慨提供。虽然该协议主要侧重于抗体标记和实时成像方面，但有关果蝇胚胎收集和注射的更详细描述，请参阅已发表的报告15,16。
1. 抗体的荧光标记
<ol><li>优选地，使用单克隆抗体或纳米抗体来获取目标蛋白。制备 1 mg/mL 或更高的抗体储备浓度。 注：在本研究中，以GFP纳米抗体（见 材料表）为例。市售的GFP纳米抗体的包装浓度为1.0 mg/mL，体积为250 μL。 此外，还利用了市售的抗体标记试剂盒（参见 材料表），该试剂盒通过琥珀酰亚胺酯反应将 Alexa Fluor 594 偶联到蛋白质的伯胺上11。重要的是，这种标记过程不会显著改变抗体浓度。</li>
	<li>通过将组分 B（在抗体标记试剂盒中提供）重悬于 1 mL 去离子水中来制备 1 M 碳酸氢钠溶液。</li>
	<li>将抗体浓度调节至1.0 mg/mL，然后加入1/10体积（ 100μL GFP纳米抗体为10μL）的1M碳酸氢钠溶液。</li>
	<li>将 110 μL 抗体混合物（来自步骤 1.3）直接加入含有 Alexa Fluor 594 染料的试管中。倒置混合（不要涡旋）并在室温下在旋转器上孵育1小时。</li>
	<li>从偶联试剂盒中组装纯化柱（参见 材料表）。准备一个 1.5 mL 树脂床（在抗体标记试剂盒中提供），并在室温 （RT） 下以 1100 x g 离心色谱柱 3 分钟，以除去树脂中多余的液体。</li>
	<li>将反应混合物（从步骤1.4开始）滴加到树脂柱的顶部，并在4°C下以1100× g 离心5分钟以收集标记的抗体。收集的抗体应呈粉红色，体积应略小于100μL。 储存在4°C的铝箔包裹或深色管中。</li>
</ol>2. 果蝇 胚胎的制备
<ol><li>将 200 只新孵化的成年 果蝇 放入塑料圆柱形笼子（直径 = 5 厘米，高度 = 8 厘米）中，雄性与雌性的比例为 1：10。用多孔金属网密封一侧用于通风，另一侧用果汁/酵母糊琼脂平板密封。</li>
	<li>在胚胎收集前三天，每 12 小时更换一次平板。这样可以同步 果蝇 产卵并提高采集效率。</li>
	<li>在注射当天，将笼子换成含有最少酵母糊的果汁盘子，并在25°C下收集胚胎1小时。如果第一轮收集没有产生足够的胚胎（<50个胚胎），则丢弃第一块板并重复此步骤进行第二轮收集，直到在1小时内产下超过100个胚胎。</li>
	<li>从笼子中取出板以停止产卵，并在25°C下再孵育2小时，以获得2-3小时的胚胎。胚胎的正确阶段对于抗体注射的成功至关重要。</li>
	<li>要去除胚胎的蛋壳，请在果汁盘中加入2mL 50%漂白剂，然后用画笔轻轻地将胚胎从盘子中取出（图2A-4）。通常，胚胎将直接放在酵母糊的顶部。在这种情况下，可以将酵母糊刷入漂白剂溶液中以收集所有胚胎。</li>
	<li>将漂浮的胚胎在50%漂白剂中孵育2分钟，并每30秒旋转一次果汁盘，以提高蛋壳去除效率。</li>
	<li>将胚胎/漂白剂混合物倒入70μm尼龙细胞过滤器中转移（图2A-7）。用水瓶彻底清洗胚胎，以去除任何残留的漂白剂和酵母膏。用纸巾完全擦干细胞过滤器，确保去除胚胎周围的多余水分。</li>
</ol>3. 胚胎对齐和干燥
<ol><li>制备5cm x 5cm x 0.5cm（宽，长，高）4%琼脂糖凝胶（图2A-9），并让凝胶冷却至室温。使用干净的剃须刀片切割1cm x 3cm x 0.5cm（宽，长，高）琼脂糖块，并将块放在载玻片上（图2A-2）。在解剖镜下检查凝胶块，确保边缘切直，表面平整干燥。</li>
	<li>使用画笔将胚胎从过滤器转移到凝胶块上。轻轻刷洗，将胚胎沿块的中线均匀地铺开。理想情况下，胚胎簇被分成单个胚胎或双峰，而不会相互接触。</li>
	<li>准备一个镊子，两条腿紧紧地粘在一起，形成一个细尖（图2A-5）。在解剖镜下，使用镊子拾取单个胚胎，并将它们沿着凝胶块的长边缘放置。对齐20-30个胚胎，确保其前后轴平行于边缘（图2C）。</li>
	<li>在24mm×50mm盖玻片（图2A-1）的中心移液10μL庚烷胶（参见材料表），并使用移液器吸头将胶水铺入0.5cm x 3 cm矩形区域。等待胶水完全干燥后再使用。</li>
	<li>将载玻片和凝胶块放在桌子的边缘，胚胎朝外。使用平头镊子（图2A-6）用胶水提起盖玻片，并将其保持在胚胎顶部，胶水面以约45度的倾斜角度朝向胚胎。 注意：轻轻地将盖玻片压在凝胶块上，使胚胎与胶水接触，然后快速释放压力并提起盖玻片。施加的张力至关重要，这样胚胎才能稳定地附着在胶水上，而不会被压得太紧而爆裂。</li>
	<li>将10μL水移液到新载玻片的中心，并将胚胎放在盖玻片上，胚胎的一面朝上（图2B）。确保使用水代替指甲油或其他粘合剂将盖玻片固定在载玻片上，因为盖玻片的这一侧将直接放置在共聚焦透镜的顶部以进行实时成像。</li>
	<li>将胚胎在干燥室（图2A-3）（见材料表）中干燥10-15分钟，直到卵黄膜起皱（图2E）。所需时间可能因房间湿度而异，应针对每种实验室条件进行实验测试。</li>
	<li>在胚条的一端移液40μL卤代烃油（27型和700型的混合物，体积比例为1：1，参见 材料表）。倾斜载玻片，直到卤代烃油覆盖胚胎的整个表面。</li>
</ol>4. 抗体注射和成像
<ol><li>使用微量移液器拉拔器准备一些注射玻璃针（参数设置见 材料表 ），并向每个针头加载 5 μL AlexaFluor 标记的抗体溶液（来自步骤 1.6）。</li>
	<li>将 25 mm x 25 mm 的盖玻片放在载玻片的顶部。移液 40 μL 卤代烃油，并沿盖玻片边缘铺开。</li>
	<li>在注射镜下，在油下将针尖对准盖玻片的边缘。调整皮泵的注射气压（见 材料表），使一个泵产生一个充满抗体的气泡。气泡直径应限制在20-50μm（图2F）。</li>
	<li>用含有油下胚胎的载玻片替换空载玻片。将注射针尖垂直对准胚胎的前后轴（图2D，G）。</li>
	<li>检查胚胎的阶段，以确保大多数胚胎已经开始细胞化但尚未开始原肠胚形成（第4阶段和第5阶段），保留为合胞体（图2F，G）。 注意：这个阶段的标志是没有任何凹槽或褶皱，并且在胚胎中心可见椭圆形的深色卵黄囊。油下胚胎阶段的形态学特征基于VolkerHartenstein 17的“果蝇胚胎发生阶段”一章。</li>
	<li>使用 X-Y 阶段操纵器将胚胎移向针头，直到尖端到达蛋黄的中心。泵送两到三次，将抗体注射到蛋黄中。当胚胎从抗体溶液中增加体积时，卵黄膜皱纹迅速消失，表明注射成功（图2G）。</li>
	<li>使用X-Y阶段操纵器在注射后将胚胎从针头上移开，并向下移动到下一个胚胎。重复步骤6，直到注射载玻片上的所有胚胎。</li>
	<li>将注射胚胎的载玻片转移到湿度室（图2A-8）。在25°C下孵育，直到达到所需的胚胎发育阶段。</li>
	<li>将 24 mm x 50 mm 盖玻片从载玻片上取下，并将其直接放入显微镜的载玻片支架中。没有胚胎的一方将面临目标。在明场照明下使用低倍率镜头定位胚胎，并切换到 40 倍或 63 倍镜头进行高分辨率荧光实时成像。</li>
</ol>

通过抗体介导的实时成像增强蛋白质可视化

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作者没有利益冲突需要声明。

该介绍的程序概述了使用定制抗体进行荧光标记并随后注射到早期 果蝇 胚胎中的专用方法。该技术有助于实时可视化少量存在的蛋白质或翻译后修饰，这些蛋白质或翻译后修饰通常难以通过传统的GFP/mCherry标记方法观察到。
在扩展该方法以在野生型和突变型胚胎之间进行定量比较时应谨慎行事。虽然在免疫荧光中，对照组和实验组之间的一抗和二抗浓度可以保持相同?...

免疫荧光是现代细胞生物学的一项基石技术，最初由 Albert Coons 开发，它能够检测其天然细胞区室的分子并表征亚细胞器或机器的分子组成1。结合基因操作，免疫荧光有助于建立现在广为接受的概念，即蛋白质定位对其功能至关重要2。除了特异性一抗和明亮的荧光染料外，该技术的成功还依赖于称为固定和透化的初步过程，该过程保留了细胞形态，固定了抗原，并增加了抗体进入细胞内区室的可及性。不可避免地，固定和透化过程会杀死细胞并终止所有生物过程3.因此，免疫荧光仅提供蛋白质生命旅程的快照。然而，许多生物过程（如细胞迁移和分裂）本质上是动态的，需要以时空分辨的方式研究蛋白质行为4,5。
为了研究生物体中的蛋白质动力学，已经开发了基于基因编码荧光蛋白（如绿色荧光蛋白 （GFP）6 和高速共聚焦显微镜）的实时成像方法。简而言之，目标蛋白可以通过基因操作与GFP7融合，然后从病毒或酵母启动子（如巨细胞病毒（CMV）8 或上游激活序列（UAS）9）异位表达。由于GFP本质上是自发荧光的，因此不需要荧光团偶联抗体来揭示靶蛋白的定位，从而绕过了固定或透化的初步过程的必要性。在过去的二十年中，已经开发了跨越整个波长光谱的荧光标签10，可以同时对多种靶蛋白进行多色实时成像。然而，与化学工程荧光染料（如AlexaFluor或ATTO）相比，这些基因编码的荧光蛋白的自发荧光在内源性启动子表达时相对较弱且不稳定，特别是在较长时间尺度的实时成像期间10。虽然这种不足可以通过过度表达荧光标记的靶蛋白来缓解，但许多具有酶活性的蛋白（如激酶和磷酸酶）如果不在生理水平上表达，会严重破坏正常的生物过程。
该协议提出了一种在实时图像设置中实现基于光稳定抗体的靶标照明的方法，基本上允许免疫荧光，而无需固定或透化过程（图1）。通过简单的基于 NHS 的伯胺反应11，可以将荧光染料（如 AlexaFluor 488 或 594）与基本上任何一抗或 GFP/HA/Myc 纳米抗体12 偶联。利用所有 果蝇 胚胎细胞在第 13 阶段共享共同细胞质的发育特征，可以在注射染料偶联抗体后实现整个胚胎的抗原结合和照明。随着 果蝇 和其他模型系统14中可用的内源性标记蛋白库的扩展，该方法可以通过揭示活组织中低丰度荧光标记蛋白和其他非荧光标记（HA/Myc标记）蛋白的动力学来潜在地扩大这些文库的应用。

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visualizing low-abundance proteins and post-translational modifications in living drosophila embryos via fluorescent antibody injection

使用 GFP（绿色荧光蛋白）和其他荧光标签对活细胞中的蛋白质进行可视化，极大地提高了对蛋白质定位、动力学和功能的理解。与免疫荧光相比，实时成像更准确地反映了蛋白质的定位，而不会因组织固定而产生潜在的伪影。重要的是，实时成像能够对蛋白质水平和定位进行定量和时间表征，这对于理解细胞运动或分裂等动态生物过程至关重要。然而，荧光标记方法的一个主要局限性是需要足够高的蛋白质表达水平才能实现成功的可视化。因此，无法检测到许多表达水平相对较低的内源性标记荧光蛋白。另一方面，使用病毒启动子的异位表达有时会导致蛋白质错定位或生理环境中的功能改变。为了解决这些局限性，提出了一种在活胚胎中利用高灵敏度抗体介导的蛋白质检测的方法，基本上无需组织固定即可进行免疫荧光。作为原理证明，在活胚胎中几乎无法检测到的内源性 GFP 标记的 Notch 受体在抗体注射后可以成功可视化。此外，这种方法适用于可视化活胚胎中的翻译后修饰 （PTM），允许检测早期胚胎发生过程中酪氨酸磷酸化模式的时间变化，并揭示顶膜下磷酸酪氨酸 （p-Tyr） 的新亚群。这种方法可以修改以适应其他蛋白质特异性、标签特异性或 PTM 特异性抗体，并且应该与其他适合注射的模式生物或细胞系兼容。该协议为低丰度蛋白质或PTM的实时成像开辟了新的可能性，而这些蛋白质或PTM以前很难使用传统的荧光标记方法进行检测。

Immunofluorescence is a cornerstone technique of modern cell biology originally developed by Albert Coons, which enables the detection of molecules at their native cellular compartments and characterization of the molecular compositions of subcellular organelles or machineries1. Coupled with genetic manipulations, immunofluorescence helps establish the now well-accepted concept that protein localization is essential for its function2. Aside from specific primary antibodies and bright fluorescent dyes, the success of this technique relies on a preliminary process named fixation and permeabilization, which preserves cellular morphologies, immobilizes antigens, and increases the accessibility of antibodies into intracellular compartments. Inevitably, the fixation and permeabilization process would kill cells and terminate all biological processes3. Therefore, immunofluorescence only provides snapshots of the life journey of proteins. However, many biological processes such as cell migration and divisions are dynamic in nature, requiring investigation of protein behaviors in a spatial-temporally resolved manner4,5.
To examine protein dynamics in living organisms, live imaging methods based on genetically encoded fluorescent proteins such as green fluorescent protein (GFP)6 and high-speed confocal microscopes have been developed. Briefly, the protein of interest can be genetically manipulated to be fused with GFP7, and then ectopically expressed from viral or yeast promoters such as cytomegalovirus (CMV)8 or upstream activation sequence (UAS)9. Because GFP is autofluorescent in nature, no fluorophore-coupled antibodies are required to reveal the localization of target proteins, which bypasses the necessity of preliminary processes of fixation or permeabilization. Over the last two decades, fluorescent tags spanning the whole spectrum of wavelength have been developed10, enabling multi-color live imaging of several target proteins at the same time. However, compared to chemically engineered fluorescent dyes such as AlexaFluor or ATTO, the autofluorescence of these genetically encoded fluorescent proteins is relatively weak and unstable when expressed from endogenous promoters, especially during live imaging over longer time scales10. While this shortfall can be mitigated by over-expressing fluorescently tagged target proteins, many with enzymatic activities such as kinases and phosphatases severely disrupt normal biological processes if not expressed at physiological levels.
This protocol presents a method that enables photostable antibody-based target illumination in a live image setup, essentially allowing immunofluorescence without the process of fixation or permeabilization (Figure 1). Through a simple NHS-based primary amine reaction11, one can conjugate fluorescent dyes such as AlexaFluor 488 or 594 with essentially any primary antibody or GFP/HA/Myc nanobody12. Taking advantage of a developmental feature that all Drosophila embryonic cells share a common cytoplasm during the syncytium stage13, one can achieve antigen binding and illumination across entire embryos after the injection of dye-conjugated antibodies. With expanding libraries of endogenously tagged proteins available in Drosophila and other model systems14, this method can potentially broaden applications of these libraries by revealing dynamics of low-abundance fluorescently tagged proteins and other non-fluorescently tagged (HA/Myc-tagged) proteins in living tissues.

作者聚焦：揭示动物形态发生研究中机械和生化信号的动力学 

通过荧光抗体注射观察活果蝇胚胎中的低丰度蛋白质和翻译后修饰

We aim to understand how mechanical and biochemical signals correlate animal morphogenesis, including the detection and the response to forces by cells and molecules. More molecules have been discovered to be mechanosensitive, functioning differently under varying levels of tension. However, the physiological context and the function of these force-sensitive events remain largely unknown.Due to the dynamic nature of force-sensitive events, our field largely relies on high-speed fluorescence imaging and time-lapse recording to capture molecular and cellular behaviors. Many fluorescently-tagged proteins are not bright enough to be imaged, and it requires spatial-temporal resolution without significant bleach. On the other hand, traditional immunofluorescence methods can only capture a snapshot of molecular and cellular fixture after fixation.This method paves the way to dynamically track the localization of many low-abundance protein receptors of major signaling pathways, such as Notch, Wnt, and the BMP pathways. Eventually, in addition to the traditional linear signaling cascades, we can pinpoint and where the signaling events occur at the subcellular scales.

为了证明抗体注射方法相对于基于荧光标签的实时成像或免疫荧光的优势，提供了两个案例研究，以表征低丰度跨膜受体Notch的动态定位，以及一种称为酪氨酸磷酸化的翻译后修饰在活胚胎中。
Notch信号转导活性在胚胎发生和成体器官稳态过程中的细胞命运决定中起主要作用18,19。在被其配体 Delta/Jagged20 激活后，?...

Watch this Scientific Journal Video about Unveiling the Dynamics of Mechanical and Biochemical Signals in Animal Morphogenesis Research at JoVE.com

该协议描述了定制的基于抗体的荧光标记和注射到早期 果蝇 胚胎中，以实现使用传统GFP / mCherry标签方法难以检测的低丰度蛋白质或翻译后修饰的实时成像。

Visualization of proteins in living cells using GFP (Green Fluorescent Protein) and other fluorescent tags has greatly improved understanding of protein ...

我们旨在了解机械和生化信号如何与动物形态发生相关联，包括细胞和分子对力的检测和响应。更多的分子被发现是机械敏感的，在不同程度的张力下功能不同。然而，这些力敏感事件的生理背景和功能在很大程度上仍然未知。由于力敏感事件的动态性质，我们的领域在很大程度上依赖于高速荧光成像和延时记录来捕捉分子和细胞行为。许多荧光标记的蛋白质不够亮，无法成像，并且需要时空分辨率而没有明显的漂白剂。另一方面，传统的免疫荧光方法只能在固定后捕获分子和细胞固定装置的快照。该方法为动态跟踪主要信号通路（如Notch、Wnt和BMP通路）的许多低丰度蛋白受体的定位铺平了道路。最终，除了传统的线性信号级联之外，我们还可以确定信号转导事件在亚细胞尺度上发生的位置。

visualizing-low-abundance-proteins-post-translational-modifications

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JoVE Journal

Developmental Biology

Visualizing Low-Abundance Proteins and Post-Translational Modifications in Living Drosophila Embryos via Fluorescent Antibody Injection

652 次观看.  SUSTech University. 我们旨在了解机械和生化信号如何与动物形态发生相关联，包括细胞和分子对力的检测和响应。更多的分子被发现是机械敏感的，在不同程度的张力下功能不同。然而，这些力敏感事件的生理背景和功能在很大程度上仍然未知。由于力敏感事件的动态性质，我们的领域在很大程度上依赖于高速荧光成像和延时记录来捕捉分子和细胞行为。许多荧光标记的蛋白质不够亮，?...