A method for micrometer resolution patterning of primary culture neurons for SPM analysis

被引:18
作者
Degenaar, P
Le Pioufle, B
Griscom, L
Tixier, A
Akagi, Y
Morita, Y
Murakami, Y
Yokoyama, K
Fujita, H
Tamiya, E
机构
[1] Japan Adv Inst Sci & Technol, Sch Mat Sci, Hokuri Ku, Tatsunokuchi, Ishikawa 9231292, Japan
[2] Univ Tokyo, Inst Ind Sci, CNRS, LIMMS,Minato Ku, Tokyo 1068558, Japan
[3] Ecole Normale Super, F-35170 Bruz, France
关键词
neuron; patterning; SPM; SNOM; SNOAM;
D O I
10.1093/oxfordjournals.jbchem.a002995
中图分类号
Q5 [生物化学]; Q7 [分子生物学];
学科分类号
071010 [生物化学与分子生物学]; 081704 [应用化学];
摘要
In this work we present a method for ultra-fine patterning of primary culture neuron cell growth, which is compatible for scanning near-field optical atomic force microscopy (SNOAM) analysis. SNOAM uses near-field optics to break the fundamental diffraction limit imposed on normal microscopy. SNOAM can achieve sub-100 nm optical resolutions, but requires transparent, open substrates. The ability to do physiological measurements on patterns of neurons, combined with ultra high resolution optical and fluorescent analysis, is useful in the study of long-term potentiation. The patterning method consists of chemical guidance with an element of physical confinement and allows for ultra-fine patterning of neural growth on transparent glass substrates. Substrates consist of microfabricated perfluoropolymer barrier structures on glass. Poly-L-lysine was selectively deposited using a silicone-based microfluidic stencil aligned to the perfluoropolymer/glass substrate. Primary culture neurons were extracted from 8-day-old chicks and grown for 3 days to form good networks. This patterning system shows very specific growth with patterning separations down to the level of individual neurites. Fluorescent imaging was carried out on both cell viability during growth and immuno-tagged microtubule-associated proteins on the neurites. Neurons inside the patterned structures were imaged and analyzed with a tapping mode SNOAM.
引用
收藏
页码:367 / 376
页数:10
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