D，L-α-二氟甲基鸟氨酸（DFMO）增强的[3H]腐胺摄取对9L肿瘤细胞生长和集落形成效率的影响。

Effect of D,L-alpha-difluoromethylornithine (DFMO) enhanced [3H]putrescine uptake on 9L tumor cell growth and colony forming efficiency.

作者信息

Redgate E S, Grudziak A, Floyd K L, Deutsch M, Boggs S S

机构信息

Dept. of Physiology, University of Pittsburgh School of Medicine, PA 15261.

出版信息

Int J Radiat Oncol Biol Phys. 1993 Mar 15;25(4):639-46. doi: 10.1016/0360-3016(93)90010-s.

DOI:10.1016/0360-3016(93)90010-s

PMID:8454482

Abstract

PURPOSE

This study explored the possible use of D,L- alpha-difluoromethylornithine (DFMO) to enhance the uptake of [3H] putrescine in order to selectively kill brain tumor cells.

METHODS AND MATERIALS

Gliosarcoma cells (9L) were grown for 4 or 20 day periods in monolayer cultures with or without [3H] putrescine and/or DFMO. Cells in culture incubated for 20 days were replated at 4-day intervals. Cells were counted on a Coulter Electronic Particle Counter and percent viability was determined by eosin dye exclusion. Survival of cells with proliferative capacity was assayed by their colony. Forming ability and surviving fraction was calculated. The radioactive counts due to [3H] putrescine were measured in 9L cells and in medium and expressed as cpm/100 cells or cpm/ml, respectively.

RESULTS

As previously reported (15), DFMO treatment resulted in termination of cell proliferation that was reversible by the addition of exogenous putrescine. Specifically, after 4 days in culture, cell counts in groups exposed to 10 mM DFMO were 55% of those in control groups and addition of 3 mM putrescine reversed the DFMO effects. Uptake of [3H] putrescine into untreated cells increased in proportion to the amount of exogenous putrescine present during 4 days of culture (range 0.01 nmol to 100 nmol) and the presence of DFMO in the medium enhanced the uptake 9 fold throughout these ranges. At activities greater than 100 cpm/100 cells the cell count was reduced to 23 to 48% of control after 4 days in culture. Extending the treatment to 20 days of incubation increased the killing of 9L cells. During the 20-day incubation, control cells increased from 5 x 10(5) to 13 x 10(12) of which 90% were colony forming cells. Treatment with either 25 microCi [3H] putrescine or 1 mM DFMO for 4 days followed by removal of these agents and incubation for an additional 16 days for a total of 20 days resulted in 31 x 10(8) or 18 x 10(7) colony forming cells, respectively. Combining [3H] putrescine and DFMO treatments during the first 4 days of the 20 day incubation reduced the colony forming cells to 21 x 10(5) (surviving fraction to 67%). When the DFMO treatment was present during the entire 20 days, it became cytotoxic since the colony forming cells were reduced to 35 x 10(3) (surviving fraction was 17%). The combination of the 4-day [3H putrescine and the 20 day DFMO treatments resulted in only 1200 surviving colony forming cells (surviving fraction was only 2%).

CONCLUSION

DFMO treatment of 9L cells for 20 days resulted in increased uptake of [3H] putrescine, a 10(10) fold inhibition of colony forming cells and extensive 9L cell killing relative to untreated controls.

摘要

目的

本研究探索了使用D，L-α-二氟甲基鸟氨酸（DFMO）来增强[3H]腐胺摄取，从而选择性杀死脑肿瘤细胞的可能性。

方法和材料

将胶质肉瘤细胞（9L）在含有或不含有[3H]腐胺和/或DFMO的单层培养物中培养4天或20天。将培养20天的细胞每隔4天重新接种。使用库尔特电子粒子计数器对细胞进行计数，并通过伊红染料排斥法测定细胞活力百分比。通过细胞集落形成能力来测定具有增殖能力的细胞的存活率，并计算存活分数。在9L细胞和培养基中测量[3H]腐胺的放射性计数，分别表示为每分钟计数/100个细胞或每分钟计数/毫升。

结果

如先前报道（15），DFMO处理导致细胞增殖终止，添加外源性腐胺可使其逆转。具体而言，培养4天后，暴露于10 mM DFMO的组中的细胞计数为对照组的55%，添加3 mM腐胺可逆转DFMO的作用。在培养4天期间（范围为0.01 nmol至100 nmol），未处理细胞对[3H]腐胺的摄取与外源性腐胺的量成比例增加，并且培养基中DFMO的存在在这些范围内将摄取增强了9倍。在培养4天后，当活性大于100 cpm/100个细胞时，细胞计数降至对照组的23%至48%。将处理延长至20天的孵育增加了对9L细胞的杀伤。在20天的孵育期间，对照细胞从5×10⁵增加到13×10¹²，其中90%是集落形成细胞。用25微居里[3H]腐胺或1 mM DFMO处理4天，然后去除这些试剂并再孵育16天，总共2０天，分别产生31×10⁸或18×10⁷个集落形成细胞。在20天孵育的前4天将[3H]腐胺和DFMO处理相结合，使集落形成细胞减少到21×10⁵（存活分数降至67%）。当在整个20天期间都存在DFMO处理时，它变得具有细胞毒性，因为集落形成细胞减少到35×10³（存活分数为17%）。4天的[3H]腐胺和20天的DFMO处理相结合仅产生1200个存活的集落形成细胞（存活分数仅为2%）。