南方医科大学学报

南方医科大学学报 ›› 2020, Vol. 40 ›› Issue (11): 1656-1661.doi: 10.12122/j.issn.1673-4254.2020.11.19

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银染法和鬼笔环肽染色观察不同发育阶段小鼠骨细胞突触

冯舒皓,包良笑,邱耿涛,廖哲霆,邓仲豪,陈纳淳,楚玉豪,骆梓恒,金 昱,李啸宇,杨英姿,赵 亮   

  • 出版日期:2020-11-20 发布日期:2020-11-23

Observation of dendrite osteocytes of mice at different developmental stages using Ploton silver staining and phalloidin staining

  • Online:2020-11-20 Published:2020-11-23

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摘要: 目的 采用银染法和鬼笔环肽染色方法探究骨细胞突触在不同发育阶段的组织形态并探讨两种染色方法在观察小鼠骨细胞不同发育阶段形态中应用价值。方法 取出生后0 dP0)、5 dP5)、15 dP15)、21 dP21)、28 dP28)、35 dP35)野生型小鼠的肱骨、股骨,制备冰冻切片及石蜡切片。对P35小鼠的股骨切片进行H&E染色,作为观察骨小梁和皮质骨中骨细胞的参照。对其他时期的肱骨组织切片采用银染法染色观察骨细胞和骨小管的形态,并记录各时期小鼠肱骨骨皮质和骨小梁中骨小管的长度。选取P10P15两个时期小鼠肱骨的冰冻切片进行鬼笔环肽 iFlour-488染色,观察骨细胞的形态,并记录骨皮质中骨细胞突触的长度。结果 通过银染法染色,在P0~P15时期的小鼠肱骨骨小梁中,我们仅能观察到骨细胞轮廓,无法观察到骨小管的形态。在P21后,通过银染法可以观察到骨小梁骨细胞及骨小管的形态,且骨细胞周围骨小管的长度随年龄逐渐变长,P21 vs P28P<0.05),P21 vs P35P<0.05),排列整齐。在P15时期的小鼠肱骨骨皮质中,通过银染法即可以观察到骨细胞及骨小管的形态,且骨细胞周围骨小管的长度随年龄逐渐变长,P15 vs P21P<0.005),P15 vs P28P<0.0001),P15 vs P35P<0.0001),排列整齐。采用鬼笔环肽iFlour-488染色,可以观察到P10P15时期骨细胞的完整形态,骨细胞突触随着年龄增加逐渐变长,P10 vs P15P<0.01),与周围骨细胞连接。结论 小鼠骨细胞突触随骨骼发育长度逐渐加长、排列逐渐整齐。银染法可以观察成年后骨细胞及骨小管的形态,对生长发育早期的骨小管形态显像不足。鬼笔环肽染色标记细胞骨架的方法适用于生长发育各时期的骨细胞染色,可以实现在发育早期对骨细胞的形态的检测。

关键词: 骨细胞, 骨小管, 银染法, 鬼笔环肽

Abstract: Objective To assess the value of Ploton silver staining and phalloidin-iFlour 488 staining in observation of the morphology of osteocyte dendrites of mice at different developmental stages. Methods The humerus and femurs were harvested from mice at 0 (P0), 5 (P5), 15 (P15), 21 (P21), 28 (P28), and 35 days (P35) after birth to prepare cryo-sections and paraffin sections. HE staining of P35 mouse femur sections served as a reference for observing osteocytes in the trabecular bone and cortical bone. The humeral sections at different developmental stages were stained with Ploton silver staining to observe the morphology of osteocytes and canaliculi, and the canalicular lengths in the cortical and trabecular bones of the humerus of the mice in each developmental stage were recorded. The cryo-sections of the humerus from P10 and P15 mice were stained with phalloidin iFlour-488 to observe the morphology of osteocytes and measurement of the length of osteocyte dendrites in the cortical bone. Results In the trabecular bone of the humerus of P0-P15 mice, Ploton silver staining only visualized the outline of the osteocytes, and the morphology of the canaliculi was poorly defined. In P21 or older mice, Ploton silver staining revealed the morphology of the trabecular bone osteocytes and the canaliculi, which were neatly arranged and whose lengths increased significantly with age (P21 vs P28, P<0.05; P21 vs P35, P<0.05). In the humeral cortical bone of P15 mice, the morphology of the osteocytes and canalicular could be observed with Ploton silver staining, and the length of the regularly arranged canaliculi of the osteocytes increased significantly with age (P15 vs P21, P<0.005; P15 vs P28, P<0.0001; P15 vs P35, P<0.0001). Phalloidin iFlour-488 staining was capable of visualizing the complete morphology of the osteocytes at P10 and P15; the osteocyte dendrites elongated progressively with age (P10 vs P15, P<0.01) to form connections with the surrounding osteocytes. Conclusion Mouse osteocyte dendrites elongate progressively and their arrangement gradually becomes regular with age. Ploton silver staining can clearly visualize the morphology of the osteocytes and the canaliculi in adult mice but not in mice in early stages of development. Phalloidin iFlour-488 staining for labeling the cytoskeleton can be applied for mouse osteocytes at all developmental stages and allows morphological observation of mouse osteocytes in early developmental stages.

Key words: osteocytes, canaliculi, Ploton silver staining, phalloidin