AtFH14 以不同的方式交联肌动蛋白丝和微管。

AtFH14 crosslinks actin filaments and microtubules in different manners.

机构信息

Key Laboratory of Cell Proliferation and Regulation Biology of Ministry of Education, Center for Biological Science and Technology, Advanced Institute of Natural Science, Beijing Normal University, Zhuhai, 519087, China.

Key Laboratory of RNA Biology, CAS Center for Excellence in Biomacromolecules, Institute of Biophysics, Chinese Academy of Sciences, Beijing, 100101, China.

出版信息

Biol Cell. 2021 May;113(5):235-249. doi: 10.1111/boc.202000147. Epub 2021 Feb 1.

DOI:10.1111/boc.202000147

PMID:33386758

Abstract

BACKGROUND INFORMATION

In many cellular processes including cell division, the synergistic dynamics of actin filaments and microtubules play vital roles. However, the regulatory mechanisms of these synergistic dynamics are not fully understood. Proteins such as formins are involved in actin filament-microtubule interactions and Arabidopsis thaliana formin 14 (AtFH14) may function as a crosslinker between actin filaments and microtubules in cell division, but the molecular mechanism underlying such crosslinking remains unclear.

RESULTS

Without microtubules, formin homology (FH) 1/FH2 of AtFH14 nucleated actin polymerisation from actin monomers and capped the barbed end of actin filaments. However, in the presence of microtubules, quantitative analysis showed that the binding affinity of AtFH14 FH1FH2 to microtubules was higher than that to actin filaments. Moreover, microtubule-bound AtFH14 FH1FH2 neither nucleated actin polymerisation nor inhibited barbed end elongation. In contrast, tubulin did not affect AtFH14 FH1FH2 to nucleate actin polymerisation and inhibit barbed end elongation. Nevertheless, microtubule-bound AtFH14 FH1FH2 bound actin filaments and the bound actin filaments slid and elongated along the microtubules or elongated away from the microtubules, which induced bundling or crosslinking of actin filaments and microtubules. Pharmacological analyses indicated that AtFH14 FH1FH2 promoted crosslinking of actin filaments and microtubules in vivo. Additionally, co-sedimentation and fluorescent dye-labelling experiments of AtFH14 FH2-truncated proteins in vitro revealed the essential motifs of bundling actin filaments or microtubules, which were 63-92 aa and 42-62 aa in the AtFH14 FH2 N-terminal, respectively, and 42-62 aa was the essential motif to crosslink actin filaments and microtubules.

CONCLUSIONS AND SIGNIFICANCE

Our results aid in explaining how AtFH14 functions as a crosslinker between actin filaments and microtubules to regulate their dynamics via different manners during cell division. They also facilitate further understanding of the molecular mechanisms of the interactions between actin filaments and microtubules.

摘要

背景信息

在包括细胞分裂在内的许多细胞过程中，肌动蛋白丝和微管的协同动力学起着至关重要的作用。然而，这些协同动力学的调节机制尚未完全了解。formin 等蛋白质参与肌动蛋白丝-微管相互作用，拟南芥formin14（AtFH14）可能在细胞分裂中作为肌动蛋白丝和微管之间的交联剂发挥作用，但这种交联的分子机制尚不清楚。

结果

没有微管时，AtFH14 的formin 同源结构域（FH）1/FH2 从肌动蛋白单体中引发肌动蛋白聚合，并在肌动蛋白丝的棘状末端封端。然而，在存在微管的情况下，定量分析表明，AtFH14 FH1FH2 与微管的结合亲和力高于与肌动蛋白丝的结合亲和力。此外，微管结合的 AtFH14 FH1FH2 既不引发肌动蛋白聚合，也不抑制棘状末端延伸。相比之下，微管结合的 tubulin 不影响 AtFH14 FH1FH2 引发肌动蛋白聚合和抑制棘状末端延伸。然而，微管结合的 AtFH14 FH1FH2 结合肌动蛋白丝，结合的肌动蛋白丝沿微管滑动和延伸，或者从微管上延伸，从而诱导肌动蛋白丝和微管的束状或交联。药理学分析表明，AtFH14 FH1FH2 在体内促进肌动蛋白丝和微管的交联。此外，体外 AtFH14 FH2 截断蛋白的共沉淀和荧光染料标记实验揭示了束状肌动蛋白丝或微管的必需模体，分别位于 AtFH14 FH2 N 端的 63-92aa 和 42-62aa，并且 42-62aa 是交联肌动蛋白丝和微管的必需模体。