185,463 research outputs found

    RECONSTITUTION OF ALLOPHYCOCYANIN FROM Mastigocladus laminosus WITH ISOLATED LINKER POLYPEPTIDE

    No full text
    The core linker polypeptide Lc 8.9 was isolated from Mastigocladus laminosus and purified on a preparative scale. A method for the reconstitution of allophycocyanin (AP)—linker complexes from isolated polypeptides was developed. The complex (αAP(βAP)3 Lc 8.9 was reconstituted and compared to (αAPβAP) and (αAPβAP)3 by sucrose density gradient ultracentrifugation, absorption, fluorescence emission and circular dichroism spectroscopy. Differences in the spectra of reconstituted and of directly isolated AP complexes are discussed

    Fine mapping of posttranslational modifications of the linker histone H1 from Drosophila melanogaster.

    No full text
    The linker histone H1 binds to the DNA in between adjacent nucleosomes and contributes to chromatin organization and transcriptional control. It is known that H1 carries diverse posttranslational modifications (PTMs), including phosphorylation, lysine methylation and ADP-ribosylation. Their biological functions, however, remain largely unclear. This is in part due to the fact that most of the studies have been performed in organisms that have several H1 variants, which complicates the analyses. We have chosen Drosophila melanogaster, a model organism, which has a single H1 variant, to approach the study of the role of H1 PTMs during embryonic development. Mass spectrometry mapping of the entire sequence of the protein showed phosphorylation only in the ten N-terminal amino acids, mostly at S10. For the first time, changes in the PTMs of a linker H1 during the development of a multicellular organism are reported. The abundance of H1 monophosphorylated at S10 decreases as the embryos age, which suggests that this PTM is related to cell cycle progression and/or cell differentiation. Additionally, we have found a polymorphism in the protein sequence that can be mistaken with lysine methylation if the analysis is not rigorous

    Linker-Directed Assembly of Twisted <i>ortho</i>-Phenylene-Based Macrocycles

    No full text
    o-Phenylene tetramers have been coassembled with linkers into macrocycles through imine condensation. Variation of linker connectivity and length allows both [1 + 1] and [2 + 2] macrocycles to be obtained, complementing (previously reported) [3 + 3] macrocycles. For the [1 + 1] macrocycles, linker length has a clear effect on o-phenylene geometry and macrocycle stability. For the [2 + 2] macrocycles, both homo- and heterochiral configurations are observed, suggesting limited communication of helix handedness in these systems

    Linker-assisted engineering of chimeric xylanase-phytase for improved thermal tolerance of feed enzymes

    No full text
    Biological enzymes are multifunctional macromolecules that can perform hundreds of reactions simultaneously. An enzyme must possess specific characteristics to meet industrial needs, such as stability over a wide pH and temperature range and high specific activity. A phytase and xylanase mixture is generally added to poultry feed to improve the bird’s health and productivity. Despite this, animal farmers have noticed no difference in productivity, and a leading cause is the high temperature at which feed is pulverized, which inactivates enzymes. A thermo-stable enzyme system can overcome these hitches. Commonly, coatings and immobilization reduce losses caused by physical-chemical factors in feed processing and digestion. To this end, we engineered the multifunctional xylanase-phytase domains on a single polypeptide fused by a helical linker. First, the ideal linker sequence was chosen by computing each selected linker’s root mean square deviation (RMSD). The selected helical linker provides sufficient structural flexibility for substrate binding and product release evaluated by molecular docking and molecular dynamic simulation studies. Furthermore, a domain-domain interaction has stabilized the bridging partners, attaining the thermal optima for xylanase and phytase at 90 °C. Even at the above-optimal temperature (100 °C), the recombinant PLX was relatively stable and retained 64.2% and 59.2% activity for xylanase and phytase, respectively, when surveyed for ten hours. So far, to this date, this is the highest degree of thermostability achieved by any recombinant phytase or xylanase. Communicated by Ramaswamy H. Sarma</p

    Linker-free Functionalization of Phosphorene Nanosheets by Sialic Acid Biomolecules

    No full text
    The importance of sialic acid on cell functions has been recently unveiled, and consequently, great attention has been paid to its interaction with tumor cells. In this line of research, we have realized phosphorene nanosheets functionalized with sialic acid molecules for biological applications with no need for another linker molecule. The formation of phosphorene sheets is feasible by using hydrogen plasma treatment and conversion of amorphous phosphorus on silicon substrates into highly crystalline nanosheets. Through immersion of these freshly prepared nanosheets into an aqueous solution containing sialic acid molecules, the formation of chemical binding between biomolecules and P atoms is initiated to form a carpet-like coverage. We have studied these structures by using Raman spectroscopy, electron microscopy, FTIR-ATR spectroscopy, and X-ray photoelectron spectroscopy. While XPS supports the passivation of sialic-activated phosphorene nanosheets (SAP) against oxidation in air or aqueous solutions, the FTIR analysis corroborates the evolution of P–O–C and P–C bonds between such biomolecules and the sheet surface. Moreover, the high-resolution TEM images demonstrate a considerable reduction in the lattice spacing from 0.32 nm for pristine phosphorene to 0.30 nm. Similarly, Raman spectroscopy depicts a shift in A2g in-plane vibrations, owing to the evolution of stress in the passivated sheets. To investigate their biocompatibility, we examined the toxicity of these bioactivated structures and observed no or little sign of toxicity. For the latter evaluation, we exploited MTT, flow cytometry, and animal models for in vivo investigations

    Degradable and Thermosensitive Microgels with Tannic Acid as the Sole Cross-Linker

    No full text
    Poly­(N-isopropylacrylamide) (PNIPAM)–tannic acid (TA) microgels were successfully prepared via surfactant-free emulsion polymerization (SFEP) at 70 °C in aqueous solution using N-isopropylacrylamide (NIPAM) as the monomer and a natural polyphenol macromolecule, TA, as the sole cross-linker. The cross-linking network of the PNIPAM–TA microgels was confirmed to contain both physical cross-linking structures formed via hydrogen-bonding interactions between TA and PNIPAM chains and chemical cross-linking structures formed via capturing the radicals of propagating polymer chains by catechol and pyrogallol groups of TA. Furthermore, TA was applied to modify the surface of hydrophobic Fe3O4 nanoparticles, leading to hydrophilic Fe3O4@TA composite nanoparticles, which were successfully used as the cross-linker to fabricate PNIPAM–Fe3O4@TA organic–inorganic hybrid microgels. The obtained PNIPAM–TA and PNIPAM–Fe3O4@TA organic–inorganic hybrid microgels had a uniform spherical shape with a relatively narrow size distribution and exhibited thermosensitive behavior and pH-tunable degradation. The PNIPAM–TA microgels were stable in the pH range of 1.3–11.1 but underwent complete degradation with pH above 11.4. The PNIPAM–Fe3O4@TA hybrid microgels were partially degraded at pH values of 1.3 and 2.1, stable in the pH range of 3.1–11.1, and underwent complete degradation at pH above 11.4. The partial degradation of PNIPAM–Fe3O4@TA organic–inorganic hybrid microgels under strong acidic conditions was attributed to the disintegration of Fe3O4 nanoparticles. The complete degradation of both microgels at pH above 11.4 was attributed to the hydrolysis of ester groups of TA under strong alkali conditions

    ATP-dependent chromatosome remodeling

    No full text
    Chromatin serves to package, protect and organize the complex eukaryotic genomes to assure their stable inheritance over many cell generations. At the same time, chromatin must be dynamic to allow continued use of DNA during a cell's lifetime. One important principle that endows chromatin with flexibility involves ATP-dependent `remodeling' factors, which alter DNA-histone interactions to form, disrupt or move nucleosomes. Remodeling is well documented at the nucleosomal level, but little is known about the action of remodeling factors in a more physiological chromatin environment. Recent findings suggest that some remodeling machines can reorganize even folded chromatin fibers containing the linker histone H1, extending the potential scope of remodeling reactions to the bulk of euchromatin

    Structural analysis of the PRD-B-C linker region.

    No full text
    <p>(A) Crystal structure of the periplakin linker domain (PDB ID 4Q28). One protomer out of four molecules in the asymmetric unit is shown. (B) Structural alignment of the N-terminal part of periplakin linker domain with PR2 of PRD-A. (C) Structural alignment of the C-terminal part of periplakin linker domain with the N-terminal PR like motif of PRD-A.</p

    Nature-Inspired Dual Purpose Strategy toward Cell-Adhesive PCL Networks: C(-linker-)RGD Incorporation via Thiol-ene Crosslinking

    No full text
    In an attempt to mimic nature’s ability to adhere cells, PCL is often coated with nature-derived polymers or its surface is functionalized with a cell-binding motif. However, said surface modifications are limited to the material’s surface, include multiple steps, and are mediated by harsh conditions. Here, we introduce a single-step strategy toward cell-adhesive polymer networks where thiol-ene chemistry serves a dual purpose. First, alkene-functionalized PCL is crosslinked by means of a multifunctional thiol. Second, by means of a cysteine coupling site, the cell-binding motif C(-linker-)RGD is covalently bound throughout the PCL networks during crosslinking. Moreover, the influence of various linkers (type and length), between the cysteine coupling site and the cell-binding motif RGD, is investigated and the functionalization is assessed by means of static contact angle measurements and X-ray photoelectron spectroscopy. Finally, successful introduction of cell adhesiveness is illustrated for the networks by seeding fibroblasts onto the functionalized PCL networks

    C-linker region of T7 RNAP.

    No full text
    <p>(A) The C-linker region (residues 251 to 296 in cartoon format) adopts different conformations in the initiation state (yellow, 1QLN, IC3), the elongation state (Pink, 1MSW, EC), and with 7 nt transcript bound (blue, 3E2E, IC7). The P266 and L266 residue is shown in stick format. The amino acids from 255 to 263 are disordered in the P266L structure (3E2E) and shown as dashed line. The direction of rotation of the linker near the hinge region is marked with arrows. The C-terminal domains (residues 300–883) of the three structures were aligned using Pymol (Molecular graphics systems). (B) Conservation of proline residue in the linker region between N-terminal domain and C-terminal domain at positions 266 and 270 in single-subunit RNAPs of phage, bacterium, and eukaryotic mitochondria. The N-terminal 1–300 amino acid sequence of T7 RNAP was used as a query in a BLAST amino acid search of the NCBI database for sequence alignment.</p
    corecore