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Measurements of forces produced by the mitotic spindle using optical tweezers

机译:用光镊测量有丝分裂纺锤体产生的力

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We used a trapping laser to stop chromosome movements in Mesostoma and crane-fly spermatocytes and inward movements of spindle poles after laser cuts across Potorous tridactylus (rat kangaroo) kidney (PtK2) cell half-spindles. Mesostoma spermatocyte kinetochores execute oscillatory movements to and away from the spindle pole for 1-2 h, so we could trap kinetochores multiple times in the same spermatocyte. The trap was focused to a single point using a 63× oil immersion objective. Trap powers of 15-23 mW caused kinetochore oscillations to stop or decrease. Kinetochore oscillations resumed when the trap was released. In crane-fly spermatocytes trap powers of 56-85 mW stopped or slowed poleward chromosome movement. In PtK2 cells 8-mW trap power stopped the spindle pole from moving toward the equator. Forces in the traps were calculated using the equation F = Q'P/c, where P is the laser power and c is the speed of light. Use of appropriate Q' coefficients gave the forces for stopping pole movements as 0.3-2.3 pN and for stopping chromosome movements in Mesostoma spermatocytes and crane-fly spermatocytes as 2-3 and 6-10 pN, respectively. These forces are close to theoretical calculations of forces causing chromosome movements but 100 times lower than the 700 pN measured previously in grasshopper spermatocytes.
机译:我们使用诱捕激光来阻止激光切割穿过多孔三指(大鼠袋鼠)肾脏(PtK2)细胞的半纺锤体后,食管上皮细胞和起重机蝇的精母细胞的染色体运动以及纺锤极的向内运动。食管间皮瘤的精子细胞动子执行往复运动,到达和离开纺锤极1-2小时,因此我们可以将同一个精子细胞多次捕获。使用63倍油浸物镜将陷阱聚焦到单点。 15-23 mW的陷波功率会导致线粒体振荡停止或减小。释放陷阱后,金刚线振荡恢复。在鹤蝇中,精母细胞的捕获功率为56-85 mW,停止或减慢了极向染色体移动。在PtK2单元中,8 mW的陷阱功率阻止了主轴磁极向赤道移动。使用公式F = Q'P / c计算陷阱中的力,其中P是激光功率,c是光速。使用适当的Q'系数,制得的极杆运动力为0.3-2.3 pN,而食管瘤精子细胞和鹤蝇精细胞的染色体运动分别为2-3 pN和6-10 pN。这些力与引起染色体运动的力的理论计算相近,但比蚱grass精细胞中先前测得的700 pN低100倍。

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