Live-cell imaging under centrifugation: New method measure the forces that keep the nuclei of living cells centered

23 Oct 2024, 20:52 by Mark Wolverton

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MBL Senior Scientists / study co-authors Michael Shribak, left, and Rudolf Oldenbourg with the ShinyaScope, a microscope invented by the late MBL Distinguished Scientist Shinya Inoue. Credit: Diana Kenney

Using two specialized microscopes invented at the Marine Biological Laboratory (MBL), a team of researchers from Japan and the MBL have developed a new method to measure the forces that keep the nucleus centered within a living cell. The experiments also provided important new clues about the properties of cellular cytoplasm and the mechanisms of organelle motion within cells. The work appears in Proceedings of the National Academy of Sciences.

"Understanding the mechanism of nuclear positioning is important in understanding cell division," a central process in the early development, growth, and health of all living organisms, says study lead author Akatsuki Kimura, professor at the Cell Architecture Laboratory at the National Institute of Genetics in Japan. "Cells must divide evenly to produce cells of the same size. For the cell to divide at the center, positioning of the nucleus at the cell center is critical."

Kimura adds that "it has been a mystery how a large structure, such as the cell nucleus, can move inside the crowded cell interior."

While it's long been known that appropriate positioning and movement of the nucleus and other organelles are crucial for cell functioning, the ability to accurately measure such intracellular forces has been limited.

Previous work on sea urchin eggs using a magnetic tweezers technique succeeded in measuring forces to move the nucleus, but the underlying mechanism of force production was not clear due to limitations on genetic experimental techniques in this species. The nematode C. elegans, which has a wealth of genetic techniques available, provides another convenient species for investigation of nuclear centering.

Rather than the magnetic tweezers method, which implants magnetic beads inside the nucleus that can be moved with an external magnet, the researchers chose a different approach: spinning the cells, because when a cell is rotated at very high speed, the nucleus is displaced from the center.

The team examined live embryos of C. elegans using two instruments invented at the MBL: the centrifuge polarizing microscope (CPM), developed by the late MBL Distinguished Scientist Shinya Inoué, and the orientation-independent differential interference contrast (OI-DIC) microscope, developed by MBL Senior Scientist Michael Shribak.

Shinya Inoue with his centrifuge polarizing microscope at the Marine Biological Laboratory in 2006.. Credit: Tom Kleindinst

The CPM applies controllable centrifugal forces to a sample by spinning it at high speeds while illuminating it with stroboscopic laser pulses. Using the CPM, Kimura, Makoto Goda (Hamamatsu University School of Medicine), Tomomi Tani (National Institute of Advanced Industrial Science and Technology, then at MBL) and MBL Senior Scientist Rudolf Oldenbourg discovered that when fertilized C. elegans eggs are centrifuged, the cell nucleus is displaced from the center of the cell.

To convert centrifugal speed into force, the research group used the OI-DIC microscope, which characterizes the mass density of the cytoplasm and the nucleus by measuring differences in refractive index, allowing calculation of the precise force acting on the nucleus.

With the CPM and OI-DIC microscopes, "we can now compare the two species [nematode and sea urchin] and discuss the generalities and differences," says Kimura.

The work revealed that the force required to move the nucleus in C. elegans was approximately one-sixth less than that measured in the sea urchin, although still larger than theoretically estimated. According to Kimura, "this means that there is an unknown property of the cytoplasm that makes large organelles difficult to move, and which is not accounted for in the current theory."

The nuclear centering mechanism is considered most likely dependent on microtubule activity within the cell, although it's still debated whether microtubules are pushing or pulling against the cell cortex. The results of this study were consistent with the latter mechanism, but further work and perhaps comparison with other research organisms will help settle the question.

"We established a new way to use the power of the CPM and OI-DIC microscopes to measure the force in C. elegans," says Kimura.

Because this new technique doesn't require the injection of beads into the cell, like the magnetic or optical tweezers method, it's less complex and more versatile. Now, says Kimura, "we can conduct the experiments in various gene-manipulated cells to reveal the relationship between physical force and genes."

More information: Makoto Goda et al, Live-cell imaging under centrifugation characterized the cellular force for nuclear centration in the Caenorhabditis elegans embryo, Proceedings of the National Academy of Sciences (2024). DOI: 10.1073/pnas.2402759121

Journal information: Proceedings of the National Academy of Sciences

Provided by Marine Biological Laboratory