[基质金属蛋白酶-2靶向可激活细胞穿透肽的特性及体外成像研究]

[Characteristics and in vitro imaging study of matrix metalloproteinase-2 targeting activable cell-penetrating peptide].

作者信息

Liu Min, Guo You-min, Wang Peng, Guo Xiao-juan, Yang Jun-le, Wang Si-cen, Duan Xiao-yi, Xu Gui-ping

机构信息

Imaging Center, The 2nd Affiliated Hospital of Medical School, Xi'an Jiao Tong University, Xi'an 710004, China.

出版信息

Zhonghua Yi Xue Za Zhi. 2007 Jan 23;87(4):233-9.

PMID:17425865

Abstract

OBJECTIVE

To study invasively imaging MMP2-positive tumor cell by paramagnetic Gadolinium or fluorescein carried by a activable cell penetrating peptides.

METHODS

To label Fluorescein-5-isothiocyanate (FITC) and gadopentetate with the activable cell-penetrating peptides by a solid-phase synthesis method. Identification by TOF mass spectrum (TOF-MS). Isoelectric point of the activable cell penetrating peptides is determined by disc electrophoresis. T1 relacion of gadopentetate labeled with the activable cell-penetrating peptides (B) in water were determined on 400 MHZ NMR. Human lung cancer cell lines: A549 were respectively stained by FITC labeled with ACPPs (A) or FITC alone. MMP2 expression and activity were determined by zymography. T1WI signal of A549 incubated with 120 nmol/ml B or Diethylenetriaminepentaacetic Acid-Gadolinium (Gd-DTPA) for different times were obtained by 1.5T MRI. The location of B in A549 was detected by Transmission Electron Microscopy. Visualization analysis and half-quantitative analysis were used to determine the signal characteristics. The ANOVA analysis and the paired samples t test were performed by SPSS 13.0.

RESULTS

MALDI TOF-MS molecular weigh of A and B respectively is 3789.74 and 3911.93. Isoelectric point is 11.005T1 Relacion of 0.5 mmol/L Gd-DTPA and B at 17 degrees C respectively is (0.052 +/- 0.01) sec and (0.050 +/- 0.001) sec. Fluorescein uptake assays showed that A translocated into A549 but would be inhibited by MMP2 antibody. Zymography showed both active-MMP2 (67000) and pro-MMP2 (72000) expressed byA549. MR imaging showed A549 incubating with B had a high T(1) signal, and the signal of A549 incubating with Gd-DTPA is similar with that of the control group. Furthermore, ANOVA suggested that the T(1) signal intensity of A549 incubating with B was effected by incubating time (F = 267.569, P < 0.001) and increasing in a time-dependent fashion at the observed time. There is no difference between the T(1) signal intensity of A549 incubating with Gd-DTPA and the control group (P > 0.05). TEM showed A in cytoplasm and nucleus.

CONCLUSION

The study in vitro suggests that the MMP-2 activable cell-penetrating peptides bearing contrast media can detect the MMP2-positive tumor cell.

摘要

目的

通过可激活细胞穿透肽携带的顺磁性钆或荧光素对MMP2阳性肿瘤细胞进行侵入性成像研究。

方法

采用固相合成法将可激活细胞穿透肽与异硫氰酸荧光素（FITC）和钆喷酸葡胺进行标记。通过飞行时间质谱（TOF-MS）进行鉴定。采用圆盘电泳法测定可激活细胞穿透肽的等电点。在400MHz核磁共振仪上测定可激活细胞穿透肽标记的钆喷酸葡胺（B）在水中的T1弛豫时间。人肺癌细胞系A549分别用ACPPs标记的FITC（A）或单独的FITC进行染色。通过酶谱法测定MMP2的表达和活性。用1.5T磁共振成像仪获取A549与120nmol/ml B或二乙三胺五乙酸钆（Gd-DTPA）孵育不同时间后的T1WI信号。通过透射电子显微镜检测B在A549中的定位。采用可视化分析和半定量分析确定信号特征。使用SPSS 13.0进行方差分析和配对样本t检验。

结果

A和B的基质辅助激光解吸电离飞行时间质谱分子量分别为3789.74和3911.93。等电点为11.005。17℃时，0.5mmol/L Gd-DTPA和B的T1弛豫时间分别为（0.052±0.01）秒和（0.050±0.001）秒。荧光素摄取试验表明，A可转运至A549中，但会被MMP2抗体抑制。酶谱法显示A549表达活性MMP2（67000）和前体MMP2（72000）。磁共振成像显示，A549与B孵育后T1信号升高，A549与Gd-DTPA孵育后的信号与对照组相似。此外，方差分析表明，A549与B孵育后的T1信号强度受孵育时间影响（F = 267.569，P < 0.001），且在观察时间内呈时间依赖性增加。A549与Gd-DTPA孵育后的T1信号强度与对照组无差异（P > 0.05）。透射电子显微镜显示A存在于细胞质和细胞核中。