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10-Azabicyclo[4.3.1]decan-3-ol, 10-methyl-, exo- | 492-50-2

中文名称
——
中文别名
——
英文名称
10-Azabicyclo[4.3.1]decan-3-ol, 10-methyl-, exo-
英文别名
10-methyl-10-aza-bicyclo[4.3.1]decane-8endo-ol;10-Methyl-10-aza-bicyclo[4.3.1]decan-8endo-ol
10-Azabicyclo[4.3.1]decan-3-ol, 10-methyl-, exo-化学式
CAS
492-50-2;89919-47-1
化学式
C10H19NO
mdl
——
分子量
169.267
InChiKey
GRTUMAPTPAESLY-MYJAWHEDSA-N
BEILSTEIN
——
EINECS
——
  • 物化性质
  • 计算性质
  • ADMET
  • 安全信息
  • SDS
  • 制备方法与用途
  • 上下游信息
  • 反应信息
  • 文献信息
  • 表征谱图
  • 同类化合物
  • 相关功能分类
  • 相关结构分类

计算性质

  • 辛醇/水分配系数(LogP):
    1.38
  • 重原子数:
    12.0
  • 可旋转键数:
    0.0
  • 环数:
    2.0
  • sp3杂化的碳原子比例:
    1.0
  • 拓扑面积:
    23.47
  • 氢给体数:
    1.0
  • 氢受体数:
    2.0

反应信息

  • 作为产物:
    描述:
    alkaline earth salt of/the/ methylsulfuric acid 在 甲醇 作用下, 60.0 ℃ 、11.77 MPa 条件下, 生成 10-Azabicyclo[4.3.1]decan-3-ol, 10-methyl-, exo-
    参考文献:
    名称:
    Improved yield and functionality of parathyroid cells separated by using collagenase-digestion with cold pre-incubation
    摘要:
    Preparation of cells from solid organs often induces a functional impairment due to the proteolytic cell damage by the applied digestive enzyme like collagenase, trypsin or dispase. To preserve the tissue and to enhance the yield of cells, Laue et al. reported an islet cell isolation with pre-incubation at 4 C permitting the enzyme to diffuse into the tissue and explicite activity equally throughout the whole particle. The aim of this study was to investigate whether this procedure can be applied to parathyroid glands. Therefore porcine parathyroid glands were dissected into 1 mm(3) pieces. Subsequently one group of these pieces was incubated 22 h at 4 C in 2 mg/ml collagenase before activating the enzyme by elevating the temperature to 37 C for 30 min. The other group was incubated directly at 37 C for 30 min. The yield of cells and their viability was assessed by light-microscopy and staining with trypan-blue. After the cells were immobilized in barium-alginate and cultivated for 7 days, the function was tested by incubation in different calcium concentrations and PTH-measurement. Finally, the viability was assessed by histology. Using a cold pre-incubation with collagenase, a significantly higher number of isolated cells was retrieved compared with collagenase-digestion without pre-incubation. The viability was about 100% and did not differ between both groups. After immobilization and cultivation the viability decreased to less than 30%, with and without pre-incubation. In contrast to viability the PTH-secretion of the cells differed significantly between both procedures. By preincubation with collagenase at 4 C a gentle method is presented resulting in an enhancement of yield and function of single cells of parathyroid glands. (C)2001, Editrice Kurtis .
    DOI:
    10.1007/bf03343821
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文献信息

  • Alder et al., Justus Liebigs Annalen der Chemie, 1956, vol. 601, p. 128,152
    作者:Alder et al.
    DOI:——
    日期:——
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