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Noninvasive measurement of the pH of the endoplasmic reticulum at rest and during calcium release

机译:静息和钙释放过程中内质网pH值的无创测量

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摘要

The pH within individual organelles of the secretory pathway is believed to be an important determinant of their biosynthetic activity. However, little is known about the determinants and regulation of the pH in the secretory organelles, which cannot be readily accessed by [H+]-sensitive probes. We devised a procedure for the dynamic, noninvasive measurement of pH in the lumen of the endoplasmic reticulum in intact mammalian cells. A recombinant form of the B subunit of Shiga toxin, previously modified to include a carboxyl-terminal KDEL sequence and a pH-sensitive fluorophore, was used for a two-stage delivery strategy. Retrograde traffic of endogenous lipids was harnessed to target this protein to the Golgi complex, followed by retrieval to the endoplasmic reticulum (ER) by KDEL receptors. Immunofluorescence and immunoelectron microscopy were used to verify the subcellular localization of the modified B fragment. Fluorescence ratio imaging and two independent calibration procedures were applied to determine the pH of the ER in situ. We found that the pH of the endoplasmic reticulum is near neutral and is unaffected during agonist-induced release of calcium. The ER was found to be highly permeable to H+ (equivalents), so that the prevailing [H+] is susceptible to alterations in the cytosolic pH. Plasmalemmal acid-base transporters were shown to indirectly regulate the endoplasmic reticulum pH.
机译:分泌途径的各个细胞器内的pH被认为是其生物合成活性的重要决定因素。然而,关于分泌细胞器中pH的决定因素和pH调节知之甚少,[H + ]敏感探针无法轻易访问这些因素。我们设计了一种程序,用于动态,无创地测量完整哺乳动物细胞内质网腔内的pH值。志贺毒素的B亚基的重组形式,经过预先修饰以包含羧基末端KDEL序列和pH敏感的荧光团,被用于两阶段传递策略。利用内源性脂质的逆行运输将该蛋白靶向高尔基复合体,然后通过KDEL受体检索到内质网(ER)。免疫荧光和免疫电子显微镜被用来验证修饰的B片段的亚细胞定位。应用荧光比成像和两个独立的校准程序来确定ER的pH。我们发现内质网的pH值接近中性,并且在激动剂诱导的钙释放过程中不受影响。发现ER对H + (当量)具有很高的渗透性,因此主要的[H + ]易受细胞质pH值变化的影响。血浆马来酸基础转运蛋白可间接调节内质网的pH。

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