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Quantification of iron-labeled cells with positive contrast in mouse brains

机译:定量测定小鼠脑中铁标记细胞的阳性对比

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Purpose: To quantify small amounts of iron-labeled cells in mouse brains with magnetic resonance imaging (MRI). Procedures: Iron-labeled cells (from 500 to 7,500) were stereotaxically transplanted into the brain of living mice that were subsequently imaged with MRI at 4.7 T. We compared four quantitative methods: (1) T2 relaxometry, (2) T2* relaxometry, (3) the volume of the cloverleaf hypointense artifact generated on T2*-weighted images, and (4) the volume of the cloverleaf hyperintense artifact generated on positive contrast images. Results: The methods based on relaxometry, whether T2 or T2*, did not correlate with the number of injected cells. By contrast, those based on measurement of cloverleaf artifact volume, whether using negative or positive enhancement, showed a significant linear relationship for the given range of cells (R [0.92-0.95], p<0.05). Conclusions: T2* artifact volume imaging (negative or positive) appears promising for the quantification of magnetically labeled cells following focal injection in the brain.
机译:目的:通过磁共振成像(MRI)定量小鼠脑中少量的铁标记细胞。程序:将铁标记的细胞(500至7,500个)立体定位移植到活体小鼠的大脑中,然后在4.7 T处进行MRI成像。我们比较了四种定量方法:(1)T2弛豫法,(2)T2 *弛豫法, (3)在T2 *加权图像上生成的苜蓿苜蓿叶形高清晰度伪像的体积,以及(4)在正对比度图像上生成的苜蓿叶苜蓿高强度的伪影的体积。结果:基于弛豫法的方法,无论是T2还是T2 *,都与注入的细胞数量无关。相比之下,基于苜蓿叶伪影量测量的结果,无论是使用负增强还是正增强,对于给定的细胞范围都显示出显着的线性关系(R [0.92-0.95],p <0.05)。结论:T2 *伪影体积成像(阴性或阳性)对于在脑部进行局部注射后对磁性标记的细胞进行量化似乎很有希望。

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