首页> 外文OA文献 >Non-invasive monitoring of physiological stress in the Western lowland gorilla (Gorilla gorilla gorilla) : validation of a fecal glucocorticoid assay and methods for practical application in the field.
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Non-invasive monitoring of physiological stress in the Western lowland gorilla (Gorilla gorilla gorilla) : validation of a fecal glucocorticoid assay and methods for practical application in the field.

机译:西部低地大猩猩(Gorilla gorilla gorilla)的生理压力的非侵入性监测:粪便糖皮质激素测定方法的验证和在该领域的实际应用方法。

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摘要

Enzymeimmunoassays (EIAs) allow researchers to monitor stress hormone output via measurement of fecal glucocorticoid metabolites (FGCMs) in many vertebrates. They can be powerful tools which allow the acquisition of otherwise unobtainable physiological information from both captive animals and wild animals in remote forest habitats, such as great apes. However, methods for hormone measurement, extraction and preservation need to be adapted and validated for field settings. In preparation for a field study of Western lowland gorillas (Gorilla gorilla gorilla) in the Central African Republic we used samples from captive gorillas collected around opportunistic stressful situations to test whether four different glucocorticoid EIAs reflected adrenocortical activity reliably and to establish the lag-time from the stressor to peak excretion. We also validated a field extraction technique and established a simple, non-freezer-reliant method to preserve FGCMs in extracts long-term. We determined the rate of FGCM change over 28 days when samples cannot be extracted immediately and over 12 h when feces cannot be preserved immediately in alcohol. Finally, we used repeat samples from identified individuals to test for diurnal variation in FGCM output. Two group-specific assays measuring major cortisol metabolites detected the predicted FGCM response to the stressor reliably, whereas more specific cortisol and corticosterone assays were distinctly less responsive and thus less useful. We detected a lag time of 2–3 days from stressor to peak FGCM excretion. Our field extraction method performed as well as an established laboratory extraction method and FGCMs in dried extracts stored at ambient temperatures were as stable as those at −20 °C over 1 yr. Hormones in non-extracted feces in alcohol were stable up to 28 days at ambient temperatures. FGCMs in un-fixed gorilla feces deteriorated to almost 50% of the original values within 6 h under field conditions. We detected no diurnal variation in FGCMs in samples from wild gorillas. Our study highlights the importance of thorough biological and immunological validation of FGCM assays, and presents validated, practical methods for the application of non-invasive adrenocortical monitoring techniques to field conservation contexts where it is crucially needed.
机译:酶免疫分析法(EIA)使研究人员可以通过测量许多脊椎动物的粪便糖皮质激素代谢物(FGCM)来监测应激激素的输出。它们可能是功能强大的工具,可让它们从边远的森林栖息地(例如大猿猴)的圈养动物和野生动物那里获取其他无法获得的生理信息。但是,激素的测量,提取和保存方法需要针对现场设置进行调整和验证。在准备对中非共和国西部低地大猩猩(Gorilla gorilla gorilla)进行实地研究时,我们使用了在机会压力情况下收集的圈养大​​猩猩的样品来测试四种不同的糖皮质激素EIA是否可靠地反映了肾上腺皮质激素活动并确定了滞后时间峰值排泄物的压力源。我们还验证了现场提取技术,并建立了一种简单的,无需冷冻的方法来长期保存提取物中的FGCM。当样品不能立即提取时,我们确定了28天之内FGCM的变化速率;当粪便不能立即保存在酒精中时,我们确定了12 h以上的FGCM变化率。最后,我们使用来自已识别个体的重复样本来测试FGCM输出的日变化。测量主要皮质醇代谢物的两个组特异性测定可靠地检测到了预测的FGCM对应激源的反应,而更特异性的皮质醇和皮质酮测定的反应明显较弱,因此使用较少。我们发现从应激源到FGCM排泄高峰的滞后时间为2-3天。我们的现场提取方法与既定的实验室提取方法一样有效,并且在室温下储存的干燥提取物中的FGCM与在-20°C下保存1年的FGCM一样稳定。酒精中未提取的粪便中的激素在环境温度下最多可稳定28天。在田间条件下,未固定的大猩猩粪便中的FGCM会在6小时内退化到原始值的近50%。我们在野生大猩猩的样本中未检测到FGCM的昼夜变化。我们的研究突出了对FGCM分析进行全面生物学和免疫学验证的重要性,并提出了经过验证的实用方法,可用于将非侵入性肾上腺皮质监测技术应用于急需的野外保护环境。

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