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使用已建立的肿瘤细胞系和新鲜肿瘤活检样本,对高效液相色谱法(HPLC)检测细胞胎盘碱性磷酸酶进行标准化及探讨其潜在用途。

Standardization and potential use of HPLC for detection of cellular placental alkaline phosphatase using established tumour cell lines and fresh tumour biopsies.

作者信息

Torabi-Pour N, Nouri A M, Chineguwndo F, Oliver R T

机构信息

Department of Medical Oncology, Royal London Hospital NHS Trust, UK.

出版信息

Urol Int. 1999;63(4):234-41. doi: 10.1159/000030457.

Abstract

Placement alkaline phosphatase (PLAP) is one of the cellular phosphatases (ALP) expressed in patients with testis cancers, particularly in seminomas. Using various techniques including Western blot and high-performance liquid chromatography (HPLC) systems and ATC2, a newly developed specific anti-PLAP monoclonal antibody (Mab), the presence of active form of PLAP in lysates prepared from testis tumour fragment and tumour cell lines, was studied. This was carried out following isolation of PLAP from biological samples using CNBr Sepharose-conjugated ATC2 beads. The results showed that: (1) The target for the newly developed Mab ATC2 was PLAP. (2) The ATC2-conjugated bead system was an efficient method for isolating pure PLAP. (3) Diethylamine (DEA), in contrast to urea and glycine, was the most efficient for separation of PLAP from ATC2-conjugated beads, as the isolated molecule did not lose any phosphatase activity and there was very little uncoupling of the ATC2 Mab from the beads. (4) ATC2-conjugated CNBr beads could pick up PLAP from a solution containing standard PLAP and lysates prepared from tumour cell lines or testis tissue fragments positive for the PLAP. (5) HPLC profile of testis tumour lines and testis tumours showed two distinct peaks with ALP activity, one at retention time 7-8 min (corresponding to 95 kDa molecule) and one at 12-13 min corresponding to 70 kDa molecule). These data demonstrated the potential use of various biochemical methods in combination with HPLC for isolation of the fully functional molecules with ALP activity from different samples including lysates prepared from patients with testis cancer. The nature of ALP activity at 95 kDa is being investigated as no such molecule has been reported previously. These techniques might have an important implication for an early detection of germ cell tumours, particularly in patients with equivocal ultrasound.

摘要

胎盘碱性磷酸酶(PLAP)是睾丸癌患者,尤其是精原细胞瘤患者体内表达的一种细胞磷酸酶(ALP)。利用多种技术,包括蛋白质免疫印迹法、高效液相色谱(HPLC)系统以及新开发的特异性抗PLAP单克隆抗体(Mab)ATC2,对睾丸肿瘤片段和肿瘤细胞系制备的裂解物中活性形式的PLAP的存在情况进行了研究。这是在使用溴化氰琼脂糖偶联的ATC2磁珠从生物样品中分离出PLAP之后进行的。结果表明:(1)新开发的Mab ATC2的靶标是PLAP。(2)ATC2偶联磁珠系统是分离纯PLAP的有效方法。(3)与尿素和甘氨酸相比,二乙胺(DEA)是从ATC2偶联磁珠中分离PLAP最有效的物质,因为分离出的分子没有丧失任何磷酸酶活性,并且ATC2 Mab与磁珠的解偶联非常少。(4)ATC2偶联的溴化氰磁珠可以从含有标准PLAP的溶液以及由PLAP呈阳性的肿瘤细胞系或睾丸组织片段制备的裂解物中提取PLAP。(5)睾丸肿瘤细胞系和睾丸肿瘤的HPLC图谱显示有两个具有ALP活性的明显峰,一个在保留时间7 - 8分钟(对应于95 kDa分子),另一个在12 - 13分钟(对应于70 kDa分子)。这些数据证明了将各种生化方法与HPLC相结合,从包括睾丸癌患者制备的裂解物在内的不同样品中分离具有ALP活性的全功能分子的潜在用途。由于此前未报道过95 kDa的ALP活性分子,目前正在对其性质进行研究。这些技术可能对生殖细胞肿瘤的早期检测具有重要意义,特别是对于超声检查结果不明确的患者。

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