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本文内容

  • 摘要
  • 摘要
  • 引言
  • 研究方案
  • 结果
  • 讨论
  • 披露声明
  • 致谢
  • 材料
  • 参考文献
  • 转载和许可

摘要

(诸多) 神经肌肉接头功能评估可以提供有关肌肉和神经之间的通信的基本信息。在这里,我们描述一项议定书,全面评估的诸多和肌肉功能使用两种不同的肌肉神经制剂,即比目鱼坐骨神经和膈肌膈。

摘要

学习运动神经元和肌肉之间的通信受损,老化和萎缩侧索硬化 (ALS) 等疾病时,神经肌肉接头 (诸多) 功能发挥了关键作用。在这里,我们描述了一个实验性的协议,可以用于衡量诸多功能相结合的电刺激的两种类型: 直接肌肉膜刺激和通过神经刺激。对这些两不同刺激的肌肉反应的比较可以帮助定义,一级功能,在诸多导致肌肉功能下降的潜在变化。

Ex vivo筹备工作适合于严谨的研究。在这里,我们描述密集的协议来衡量的肌肉和诸多功能为比目鱼坐骨神经制备和膈肌膈神经编写几个参数。议定书 》 持续约 60 分钟,进行不间断地定制抽搐动力学性质、 力频率关系的肌肉和神经的刺激和两个参数特定于诸多功能,即神经递质失败和 intratetanic 疲劳的措施的软件。这种方法用于检测损害比目鱼肌和膈膜肌肉神经制剂中通过使用 SOD1G93A转基因小鼠,ALS 无所不在 overexpresses 突变体的抗氧化剂酶超氧化物歧化酶 1 (SOD1) 实验模型。

引言

神经肌肉接头 (诸多) 是由肌肉纤维运动终板和运动神经元轴突末端之间的连接形成化学突触。诸多已被证明至关重要的作用,当肌肉和神经之间的通信是受损,发生在老化或萎缩侧索硬化 (ALS)。肌肉和神经沟通双向方式12,能够衡量诸多缺陷分别从肌肉缺损可提供其病理相互作用的新见解。事实上,这个功能的评价可能有助于评估是否形态或生化改建减少神经传递信号的功能。

作为间接测量的诸多功能,提出了肌肉收缩反应诱发神经刺激和诱发其膜的直接刺激同一块肌肉的反应的比较。事实上,自膜刺激通过传递神经传递信号,任何两个收缩反应的差异可归因于诸多的变化。这种方法已经被广泛提出大鼠34567,并也用于在鼠标模型89101112上收集信息。

在这里,我们描述详细的消费税和测试两种肌肉神经制剂,即的比目鱼坐骨神经和膈肌膈筹备工作的过程。使用定制软件,我们设计了一个连续的测试协议,结合测量的几个重要参数表征诸多和肌肉的功能,从而产生诸多损害综合评价分别从那肌肉。特别是,议定书 》 的措施抽搐力、 肌肉动力学、 直接力频率曲线和神经刺激,神经递质失败13射击和破伤风的频率,和 intratetanic 疲劳7

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研究方案

All the animal experiments were approved by the ethics committee of Sapienza University of Rome-Unit of Histology and Medical Embryology and were performed in accordance with the current version of the Italian Law on the Protection of Animals.

1. Experimental set-up

  1. Set-up the experimental system composed of 1 actuator/transducer, 2 stimulators, 1 in-vitro muscle apparatus, 1 preparatory tissue bath, 1 suction electrode, 1 digital oscilloscope, 1 stereomicroscope, 1 cold light illuminator, 1 acquisition board, 1 connector block and a personal computer.
    NOTE: Here the command software was programmed in LabView and was designed to guarantee high flexibility, accuracy, and repeatability of the stimulations. For each stimulation, the user can select the pulse width, frequency, duration, and decide whether it is delivered to the membrane or through the nerve. The user can also select the length of the rest period before each stimulation.

2. Evaluations of the NMJ contractile properties of soleus and diaphragm muscles

  1. System warm-up
    1. Prepare the Krebs Ringer buffer14 and place it in a bath of the mounting apparatus and the preparatory tissue bath. Place a 60 mm dish prepared with 4 ml of silicon in the preparatory tissue bath.
    2. Turn on the circulating water bath and set the temperature to 30 °C for the soleus muscle and to 27 °C for the diaphragm muscle.
    3. Allow 95% O2 - 5% CO2 mixture to flow into both the baths.
    4. Turn on the actuator/transducer and the two pulse stimulators and set the current values to 300 mA for membrane stimulation and to 5 mA for nerve stimulation.
      NOTE: The 300 mA current value has previously been shown not to induce any significant contraction on the nerve branches when D-tubocurarine is added to the solution15. The 5 mA current value corresponds to the amount of current required to stimulate the muscle through the nerve without creating an overlap with the membrane stimulation induced by means of the solution. Since the distance between the suction electrode and the muscle is dependent on the nerve length, this current value must be carefully adjusted before each experiment, as described below.
  2. Soleus and diaphragm dissection
    1. Sacrifice the mouse by cervical dislocation to minimize suffering, and immediately excise the muscles for testing as follows.
    2. Soleus-sciatic preparation, dissection, and set-up
      1. Spray 70% ethanol on the mouse leg and remove the skin covering the leg. Make an incision in the upper part of the leg with a pair of scissors and then pull the skin firmly. Isolate the Achilles' tendon from the tibia and then cut the Achilles' tendon with a pair of scissors.
      2. Tightly clamp the tendon with a pair of forceps and gently pull the gastrocnemius muscle together with the soleus. Once the proximal tendon of the soleus is exposed, cut the entire calf with a pair of scissors while still holding the Achilles' tendon. Immediately place the tissue sample in the preparatory tissue bath.
      3. Place the preparatory bath under the stereomicroscope and fix the calf to the silicon dish using 0.20 mm diameter stainless steel pins. Using a pair of forceps clamp the proximal tendon of the soleus and gently pull it to expose the sciatic innervation.
      4. Once the innervation is exposed (Figure 1), carefully remove the surrounding tissue to expose about 5 mm of the nerve. Use a fine pair of scissors to cut the nerve. While tightly clamping the soleus on the proximal tendon with a pair of forceps, pull it again and excise it by cutting the Achilles' tendon with a pair of scissors.
      5. Pass a nylon wire through the hole of the lever arm of the actuator/transducer. Create a noose at the end of the wire and grasp the Achilles' tendon before pulling the wire back until the muscle reaches the bath of the mounting apparatus. Clamp the proximal tendon within the fixed clamp and tie the nylon wire around the lever arm. Allow the muscle to equilibrate in the solution.
      6. Determine the initial optimal length (L0).
        1. First, stretch the muscle to preload it at 10 mN (this value guarantees the maximum twitch force (based on experience)). Then, gently stretch the muscle to change the preload and stimulate it with a series of single pulses. The optimal length is achieved when the maximum twitch force is measured.
    3. Diaphragm-phrenic preparation, dissection, and set-up
      1. Spray 70% ethanol on the mouse skin. Remove the skin covering the diaphragm muscle by making an incision over the sternum with a pair of scissors and by pulling the skin firmly.
      2. With a pair of scissors, cut the abdomen horizontally below the sternum and gently remove the intestine and the organs with a pair of forceps. Use a pair of thick scissors to cut the spine.
      3. Cut the ribs about 1 cm over the sternum and proceed horizontally. Gently remove the outer organs with a pair of forceps and cut the spine to obtain a circular ring of ribs containing the diaphragm.
      4. Wash the preparation in a dish containing the Krebs Ringer buffer and then place it in the silicon dish inside the preparatory tissue bath, with the upper side facing up and the sternum facing forward.
      5. Using the stereomicroscope, carefully remove the lungs and the remaining organs; the phrenic nerve will be visible on the right side (Figure 2A).
      6. Trim the ribs to leave a ring of about 2 mm all along the diaphragm.
      7. Using forceps, fix one 0.20 mm diameter stainless steel pin on the diaphragm central tendon at the point corresponding to the phrenic nerve innervation, and another pin on the ribs on the same axis to identify the diaphragm strip of interest.
      8. Fix two additional pins on the central tendon and another two pins on the ribs on either side of the selected strip to lay out the diaphragm. If necessary, clean the phrenic nerve from the surrounding connective tissue using forceps.
      9. Using a curved blade, cut the diaphragm on either sides of the innervation to identify a tendon-muscle-rib strip as shown in Figure 2B.
      10. Pass a nylon wire through the hole of the lever arm of the actuator/transducer. Create a noose at the end of the wire and grasp the tendon before pulling the wire back until the muscle reaches the bath of the mounting apparatus.
      11. Clamp the ribs within the fixed clamp and tie the nylon wire around the lever arm.
      12. Allow the muscle to equilibrate in the solution and determine the initial optimal length (L0).
        1. Stretch the muscle to preload it at 5 mN. Gently stretch the muscle to change the preload and stimulate it with a series of single pulses. The optimal length is achieved when the maximum twitch force is measured.

figure-protocol-7442
Figure 1 - Soleus-sciatic nerve preparation. Soleus-sciatic nerve during surgical operation for the functional tests. The sciatic is exposed using a pair of forceps. Please click here to view a larger version of this figure.

figure-protocol-7941
Figure 2 - Diaphragm-phrenic nerve preparation. Picture shows a phase of the diaphram-phrenic nerve preparation excision (A) and the strip to be mounted for functional tests (B). Please click here to view a larger version of this figure.

  1. Measuring NMJ properties separately from muscle contractility
    1. Set the best current intensity for the stimulation trough the nerve and verify that the current pulses delivered through the suction electrode do not elicit muscle contraction by the spread of current in the bath.
      1. Place the suction electrode near the muscle and pull the nerve in. While gently increasing the current intensity (starting from 5 mA), stimulate the muscle with a series of single pulses. The optimal current value is determined when the twitch force is maximum.
      2. Push the nerve out of the electrode and deliver a few single pulses. Ensure that the muscle does not contract due to overlap with the membrane stimulation by means of the solution. Pull the nerve in again.
    2. Launch the program and select the input file to run the desired testing protocol.
      NOTE: The input file includes all the stimulation parameters needed to run the entire protocol. Although the same protocol structure is used for the two muscles the stimulation parameters differ depending on the protocol refers to the soleus or diaphragm muscles.
      1. Soleus-sciatic nerve stimulation (see Table 1)
        1. Use the following pulse widths for all the electrical stimulations: 1.4 ms for sciatic nerve stimulation and 0.1 ms for direct soleus stimulation. The full protocol lasts approximately 65 min.
      2. Diaphragm-phrenic nerve stimulation (see Table 2)
        1. Use the following pulse widths for all the electrical stimulations: 1.8 ms for phrenic nerve stimulation and 0.2 ms for direct diaphragm stimulation. The full protocol lasts approximately 55 min.
      3. At the end of the experimental protocol, measure the length and the wet weight of the muscle using an analog caliper with an 0.05 mm accuracy and a precision scale with an 0.1 mg accuracy, respectively.
        1. Compute the cross sectional area (CSA) by dividing the muscle mass by the product of optimal fiber length (Lf) and the density of mammalian skeletal muscle (1.06 mg/mm3)16.
          NOTE: Lf is obtained by multiplying L0 by the fiber length/muscle length ratio (0.71 for soleus muscle16 and 1 for the diaphragm muscle17).
Type of experimentFrequencyDurationRepetitionsMuscle or Nerve stimulationPurpose
(Hz)(s)
TwitchSingle pulse1MuscleTwitch force and kinetics
Rest30
TwitchSingle pulse1Nerve
Rest30
TwitchSingle pulse1Muscle
Rest30
TwitchSingle pulse1Nerve
Rest120
Unfused tetanus400.81NerveForce/frequency curves for nerve and muscle stimulations
Rest180
Unfused tetanus600.81Muscle
Rest180
Fused tetanus800.81Nerve
Rest180
Unfused tetanus200.81Muscle
Rest180
Unfused tetanus600.81Nerve
Rest180
Fused tetanus800.81Muscle
Rest180
Unfused tetanus200.81Nerve
Rest180
Unfused tetanus400.81Muscle
Rest300
Fatigue paradigm350.81 muscle stimulation followed by 14 nerve stimulations with a rest time of 1.2 s each, repeated 20 timesNeurotransmission failure (NF)
Rest900
Fatigue paradigm800.81 muscle stimulation followed by 14 nerve stimulations with a rest time of 1.2 s each, repeated 20 timesNeurotransmission failure (NF) and Intratetanic fatigue (IF)

Table 1 - Soleus-sciatic nerve stimulation protocol. The table lists the sequence of tests that form the complete protocol for testing soleus-sciatic nerve preparations.

Type of experimentFrequencyDurationRepetitionsMuscle or Nerve stimulationPurpose
(Hz)(s)
TwitchSingle pulse1MuscleTwitch force and kinetics
Rest30
TwitchSingle pulse1Nerve
Rest30
TwitchSingle pulse1Muscle
Rest30
TwitchSingle pulse1Nerve
Rest120
Unfused tetanus600.51NerveForce/frequency curves for nerve and muscle stimulations
Rest120
Fused tetanus1000.51Muscle
Rest180
Unfused tetanus400.51Nerve
Rest120
Unfused tetanus200.51Muscle
Rest120
Unfused tetanus800.51Nerve
Rest150
Unfused tetanus800.51Muscle
Rest150
Unfused tetanus200.51Nerve
Rest120
Fused tetanus1000.51Muscle
Rest150
Fused tetanus1000.51Nerve
Rest180
Unfused tetanus600.51Muscle
Rest300
Fatigue paradigm350.331 muscle stimulation followed by 14 nerve stimulations with a rest time of 0.67 s each, repeated 20 timesNeurotransmission failure (NF)
Rest900
Fatigue paradigm800.331 muscle stimulation followed by 14 nerve stimulations with a rest time of 0.67 s each, repeated 20 timesNeurotransmission failure (NF) and Intratetanic fatigue (IF)

Table 2 - Diaphragm-phrenic nerve stimulation protocol. The table lists the sequence of tests that form the complete protocol for testing diaphragm-phrenic nerve preparations.

3. Data analysis

NOTE: At the end of the protocol compute all the desired parameters as follow.

  1. From single pulse stimulation
    1. Compute twitch force (mN; maximum active force generated during twitch) and specific twitch force (mN/mm2). Compute it by subtracting the initial preload value to the maximum force generated by the muscle. Compute the specific twitch force as twitch force divided by the muscle CSA.
    2. Compute time to peak tension (TTP) (ms) as the time from pulse release to twitch force.
    3. Compute half relaxation time (1/2RT) (ms) as the time from twitch force to 50% of twitch force.
    4. Compute dF/dt (mN/ms) as the maximum value of force derivative during the contractile phase.
    5. Compute -dF/dt (mN/ms) as the maximum value of force derivative during the relaxing phase.
  2. From pulse train stimulations
    1. Compute unfused force (mN) and specific unfused force (mN/mm2). Compute it by subtracting the initial preload value to the maximum force generated by the muscle. Compute the specific unfused force as the unfused force divided by the muscle CSA.
      NOTE: The unfused force is the maximum active force generated during a pulse train with a frequency lower than the tetanic frequency.
    2. Compute tetanic force (mN) and specific tetanic force (mN/mm2); the maximum force is the maximum active force generated during a pulse train delivered at tetanic frequency. Compute it by subtracting the initial preload value to the maximum force generated by the muscle. Compute the specific tetanic force as the tetanic force divided by the muscle CSA.
    3. Compute force-frequency curve. Plot the value of force (or specific force) obtained for each stimulation versus the increasing frequency of stimulation. Typically, it begins with the single pulse stimulation and ends up with the tetanic frequency.
  3. From fatigue paradigms
    1. Calculate neurotransmission failure (NF) as:
      figure-protocol-20879
      where MF is the force decrease following muscle stimulation and F is the force decrease following nerve stimulation, measured on the first pulse train after muscle stimulation.
    2. Calculate intratetanic fatigue (IF) as:
      figure-protocol-21191
      where Flp is the force generated by the muscle at the last pulse of stimulation, and Fm is the maximum force generated by the muscle during the same pulse train. Regarding to the nerve stimulation, compute the intratetanic fatigue on the first pulse train immediately after the direct stimulation.

4. Statistical analysis

NOTE: The statistical analysis models must be chosen according to whether muscle response to both nerve and membrane stimulations is compared within the same animal model or between 2 different animal models18,19.

  1. Use the Student's t test for TTP, 1/2RT, dF/dt, -dF/dt if comparing only muscle responses to direct and indirect stimulations. If comparing muscle preparations obtained from 2 different mouse strains, use 2-way ANOVA with stimulation type and mouse strain as fixed factors. When the 2-way ANOVA returns a significant outcome, use multiple comparison tests to search for statistical differences.
  2. For force-frequency curve (if comparing only muscle responses to direct and indirect stimulations), use 2-way ANOVA with stimulation type and frequency of stimulation as fixed factors. Use multiple comparison tests if required.
    1. If comparing muscle preparations obtained from 2 different mouse strains, use 3-way ANOVA with stimulation type, frequency of stimulation and mouse strain as fixed factors.
      1. When the 3-way ANOVA yields a significant effect of the factors animal strain and stimulation type, use 2-way ANOVA to identify significant differences between 2 groups at a time. For example, differences between the muscle response of the 2 groups to membrane stimulation, or between muscle response to direct and indirect stimulations within one group can be assessed.
  3. Intratetanic fatigue
    NOTE: Since the protocol was designed to induce fatigue in response to nerve stimulation even in control mice, this parameter can only be used to investigate differences between 2 mouse strains, and a statistical analysis within a single group would always yield significant differences.
    1. To compare two groups, use 3-way ANOVA with stimulation type, time, and mouse strain as fixed factors. When the 3-way ANOVA yields a significant effect of the factors animal strain and stimulation type, use 2-way ANOVA to identify significant differences between 2 groups at a time, as for the force-frequency curve.
  4. For neurotransmission failure, use 2-way ANOVA with animal strain and time as fixed factors. If it returns significant outcomes, use multiple comparison tests to search for statistical differences.
    NOTE: Since this parameter only returns one value for each mouse strain, it allows different mouse models to be compared.
  5. For muscle weight, length, and CSA, use Student's t test to investigate differences when comparing muscle-nerve preparations from different animal models.

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结果

我们描述了议定书 》 提供了几种神经肌肉疾病或衰老骨骼肌功能失神经支配有关的信息。这个协议可以用于确定是否 (以及,如果是这样,在哪个层面) 肌肉变化是发生在本身的肌肉或神经肌肉传递的选择性变化。如下图所示的数据是工作的以前由我们组18,肌萎缩侧索硬化疾病20结束阶段 SOD1G93A转基因小鼠模型上进行的结果...

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讨论

上述实验协议提供一个理想的测量和识别任何功能的改变发生在肌肉中直接或间接在神经肌肉接头处一级途径。由于这项技术基于间接测量的诸多功能,它不能用于建立与形态学变化或与生化指标的变化,是否有关任何缺陷。与此相反的是,它提供确定是否任何形态或生化改建有减少神经递质信号功能的有效途径。然而,力测量完成后,肌肉可以从浴、 涂抹、 在最佳长度固定,,包围嵌入化合?...

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披露声明

作者没有透露。

致谢

在作者的实验室的工作被支持基金会罗姆人和节目 (给予。GGP14066)。

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材料

NameCompanyCatalog NumberComments
Dual-Mode Lever System Aurora Scientific Inc.300Bactuator/transducer
High-Power Bi-Phase Stimulator Aurora Scientific Inc.701Bpulse stimulator (nerve)
High-Power Bi-Phase Stimulator Aurora Scientific Inc.701Cpulse stimulator (muscle)
In vitro Muscle Apparatus Aurora Scientific Inc.800A
Preparatory tissue bathRadnoti158400
Monopolar Suction ElectrodeA-M Systems573000with a home-made reference 
Oscilloscope TektronixTDS2014
StereomicroscopeNikonSMZ 800
Cold light illuminator Photonic OpticsPL 3000
Acquisition boardNational InstrumentsNI PCIe-6353
Connector blockNational InstrumentsNI 2110
Personal computerAMD Phenom II x4 970Processor 3.50 Ghz with Windows 7
LabView 2012 softwareNational Instruments
Krebs-Ringer Bicarbonate Buffer Sigma-AldrichK4002 physiological buffer
Sodium bicarbonateSigma-AldrichS5761 
Calcium chloride CaCl2Sigma-AldrichC4901anhydrous, powder, ≥97%
Buffer HEPESSigma-AldrichH3375≥99.5% (titration)
Dishes 60mm x 15mmFalcon353004Polystyrene
SiliconeSylgard 184 Silicone Elastomer Kit  0.5Kg.
ThermostatDennerleDigitalDuomat 1200
PumpNewa MiniMN 606for aquarium
Heat resistance ThermocableLucky Reptile61403-150/60Hz 50W
Bucketany 10 litersPolypropylene
O2 + 5%CO2siadMix gas
#5 Forceps Fine Science Tools11252-202 items
Spring Scissors - 8 mm BladesFine Science Tools15024-10nerve excision
Sharp Scissors Fine Science Tools 14059-11muscle removal
Delicate ScissorsWagner02.06.32external of the animal
Student Scalpel Handle #3Fine Science Tools 91003-12 
Scalpel Blades #10Fine Science Tools 10010-00
Scalpel Blades #11Fine Science Tools 10011-00
nylon wire Ø0.16 mmany

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