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Blood, 15 May 2008, Vol. 111, No. 10, pp. 4839.
Fibrin formation on fast forwardISTITUTO NAZIONALE PER LA RICERCA SUL CANCRO (IST), GENOVA, ITALY
Fibrin gel, a 3-dimensional network of fibers constituting the scaffold of the hemostatic plug, is rapidly formed following fibrinogen activation during blood coagulation. In this issue of Blood, Chernysh and Weisel provide the first direct glimpse of the fibrin polymerization process under near-physiological conditions using deconvolution microscopy.
In the meantime, in this issue of Blood, Chernysh and Weisel present an innovative study using an established but lesser-known technique, deconvolution microscopy, to image plasma clotting after spiking it with fluorescently labeled fibrinogen. Relying on a mathematical treatment of images to remove out-of-focus light from other parts of the sample so that a clear picture of a single focal plane can be obtained, this technique affords real-time monitoring of the process while avoiding the bleaching problems and the relative slowness that affect confocal microscopy. Quantitative analysis of the evolving gel parameters, like fiber lengths and branch points, can then be carried out. Furthermore, although the technique's spatial resolution does not allow the direct measurement of fiber diameters, by measuring the fluorescent intensity changes along the forming fibers, their mass can also be monitored and compared with the results of parallel turbidimetry experiments.
Examining the paper, it is difficult to resist first having a peek at the supplemental videos (available on the Blood website). At low magnification (Video S1, 10x objective), nothing apparently goes on for the first 10 seconds (corresponding to Incidentally, a rough calculation of the diffusion coefficient expected for rigid (proto)fibrils 10 to 15 µm long and 10 to 20 nm thick yields approximately 10 to 20 µm2 per minute, in the same ballpark as the observed movements. Intriguing quantitative analyses of the data are then presented by the authors, revealing details that could not be inferred from bulk techniques alone. In particular, while this study definitively confirms that the abrupt transition in the turbidity profiles is directly linked to lateral thickening, there is still a fraction of fibers that continue to grow in length and branch after the gel point, contradicting some models of fibrin polymerization predicting that the entire scaffold is laid down by the clotting time. Whether these features are directly linked to the system used to initiate the reaction (citrated plasma plus CaCl2 and tissue factor), mimicking the physiological situation, or are an intrinsic property of fibrin formation, must be elucidated in further studies. Waiting for the sequel, we are left with plenty of new evidence that fibrin assembly is a truly dynamic process requiring continued research and more detailed modeling than previously thought.
Footnotes
Conflict-of-interest disclosure: The author declares no competing financial interests.
References
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| Copyright © 2008 by American Society of Hematology Online ISSN: 1528-0020 | |||||||||
12.5 minutes reaction time), and then the 3D network rapidly blooms in flower-like fashion, pervading the entire field in the last 6 seconds (