Imbert M, Chabardès D, Montégut M, Clique A, Morel F
Pflugers Arch. 1975;354(3):213-28. doi: 10.1007/BF00584645.
A method is described, which allows adenylate cyclase activity measurement in single pieces of various nephron segments. Tubular samples of 0.5 to 2 mm length were isolated by microdissection from collagenase treated slices of rabbit kidney. A photograph of each piece was taken in order to measure its length. After a permeabilisation treatment involving preincubation in a hypoosmotic medium and a freezing step, each sample was incubated for 30 mm at 30 degrees C in a medium containing high specific (alpha-32-P)-ATP 3-10-4 M, final volume 2.5 mu 1. The (32P)-cAMP formed was separated from the other labelled nucleotides by filtering the incubate on a dry aluminium oxide microcolumn, 3H cAMP was added as a tracer for measuring cAMP recovery. The sensitivity of the method was found to be a few fentomoles (10-15 M) cAMP. cAMP generation increased linearly as a function of the incubation time up to more than 30 min, and as a function of the length of the segment used. Control and fluoride (5 mM) stimulated adenvlate cyclase activities were measured in the following segments of the nephron: early proximal convoluted tubule (PCT), pars recta of the proximal tubule (PR), thin descending limb of the loop (TDL), cortical portion of the thick ascending limb (CAL), distal convoluted tubule (dct), first branched portion of the collecting tubule (BCT), further cortical (CCT) and medullary (MCT) portions of the collecting tubule. Mean control adenylate cyclase activity varied from 7 (PR) to 75 (BCT) fmoles/mm/30 min. Flouride addition resulted in a 10 (BCT) to 50 (PR) fold increase in enzyme activity. Series of replicates gave a scatter equal to plus or minus 20% (S.D. as a per cent of the mean). The method described appears to be suitable to determine which nephron segments contain hormone-dependent adenylate cyclase.
本文描述了一种方法,该方法可用于测量各个肾单位节段单个片段中的腺苷酸环化酶活性。通过显微解剖从经胶原酶处理的兔肾切片中分离出长度为0.5至2毫米的肾小管样本。拍摄每个片段的照片以测量其长度。在经过低渗介质预孵育和冷冻步骤的通透处理后,将每个样本在含有高比活(α-32-P)-ATP 3×10⁻⁴ M、终体积2.5微升的介质中于30℃孵育30分钟。通过在干燥的氧化铝微柱上过滤孵育物,将形成的(³²P)-cAMP与其他标记核苷酸分离,加入³H cAMP作为示踪剂以测量cAMP回收率。发现该方法的灵敏度为几飞摩尔(10⁻¹⁵ M)cAMP。cAMP生成量随孵育时间延长至超过30分钟呈线性增加,并随所用节段长度增加而增加。在肾单位的以下节段中测量了对照和氟化物(5 mM)刺激的腺苷酸环化酶活性:近端小管起始段(PCT)、近端小管直部(PR)、髓袢细降支(TDL)、髓袢粗升支皮质部(CAL)、远端小管曲部(dct)、集合小管第一分支部(BCT)、集合小管进一步的皮质部(CCT)和髓质部(MCT)。对照腺苷酸环化酶平均活性从7(PR)至75(BCT)飞摩尔/毫米/30分钟不等。添加氟化物导致酶活性增加10(BCT)至50(PR)倍。一系列重复实验的离散度为正负20%(标准差占平均值的百分比)。所描述的方法似乎适用于确定哪些肾单位节段含有激素依赖性腺苷酸环化酶。
