Imaging biological structures with the cryo atomic force microscope.
AUTOR(ES)
Zhang, Y
RESUMO
It has long been recognized that one of the major limitations in biological atomic force microscopy (AFM) is the softness of most biological samples, which are easily deformed or damaged by the AFM tip, because of the high pressure in the contact area, especially from the very sharp tips required for high resolution. Another is the molecular motion present at room temperature due to thermal fluctuation. Using an AFM operated in liquid nitrogen vapor (cryo-AFM), we demonstrate that cryo-AFM can be applied to a large variety of biological samples, from immunoglobulins to DNA to cell surfaces. The resolution achieved with cryo-AFM is much improved when compared with AFM at room temperature with similar specimens, and is comparable to that of cryo-electron microscopy on randomly oriented macromolecules. We will also discuss the technical problems that remain to be solved for achieving even higher resolution with cryo-AFM and other possible applications of this novel technique.
ACESSO AO ARTIGO
http://www.pubmedcentral.nih.gov/articlerender.fcgi?artid=1233685Documentos Relacionados
- Phase imaging of moving DNA molecules and DNA molecules replicated in the atomic force microscope.
- Measuring the viscoelastic properties of human platelets with the atomic force microscope.
- Thy-1 immunolabeled thymocyte microdomains studied with the atomic force microscope and the electron microscope.
- Motion and enzymatic degradation of DNA in the atomic force microscope.
- Imaging soft samples with the atomic force microscope: gelatin in water and propanol.
