Chitin synthase localization in the diatom Thalassiosira pseudonana

Chitin constitutes an abundant component in many biologically formed minerals (biominerals). While the role of chitin for the formation and properties of calcium-based biominerals has been extensively studied, little is known about its role in silica-based biominerals. Furthermore, there is hardly any information about the enzyme machinery for chitin biosynthesis in biomineral-forming organisms. Here we have identified a chitin synthase, chs7305, in the diatom Thalassiosira pseudonana. In stationary cells, chs7305 is located specifically in a ring pattern in the region of the silicified girdle bands. The expression pattern of the chs7305 gene and the co-localization of the encoded enzyme with chitin provides evidence for the importance of chitin synthesis for cell wall function under nutrient limited conditions. Chs7305 is the first chitin synthase that has been localized in a diatom.

Diatoms are outstanding examples of unicellular organisms capable of forming complex shaped cell walls made of silica [1, 2]. The silica building blocks of the cell wall are produced in a yet little understood morphogenetic process that is believed to involve long chain polyamines (LCPA), unique families of proteins (e.g., silaffins, silacidins), and insoluble organic matrices [3, 4]. Three types of insoluble organic matrices were recently identified as integral components of the silica cell wall of the diatom Thalassiosira pseudonana: meshworks [5], microrings [6] and microplates [7]. The meshworks are chitin-based with proteins as minor components, whereas the microrings and microplates are mainly composed of proteins [5,6,7]. Many different organisms employ insoluble organic matrices as central components for the biosynthesis of mineralized structures (biomineralization) [8]. The presence of chitin is particularly well studied in CaCO₃ biomineralization [8,9,10,11,12]. In nacre it contributes to high impact resistance and is believed to influence the process of biomineralization [13, 14]. In some centric diatoms, chitin is present as crystalline β-chitin fibers that are extruded through specialized openings in the cell wall called fultoportulae. These chitin fibers are not involved in silica biomineralization, and instead are believed to slow-down the sinking rate of the photosynthetically active diatom cells by increasing their drag in the water [15,16,17]. Distinct from the chitin fibers are the chitin meshworks, which are tightly associated with the silica of the cell wall (rather than being extruded) suggesting a possible involvement in silica biogenesis [5, 18].

Potential chitin synthase genes seem to be widely distributed among diatoms and can even be found in species not known to produce extracellular chitin fibers [18]. T. pseudonana possess four potential chitin synthase genes [18, 19], which is consistent with the need to produce at least two different types of chitin, secreted fibers and silica-associated meshworks. Based on the amino acid sequence, it is impossible to predict which chitin synthase produces which type of chitin. To obtain information of the chitin synthases, we attempted the localization of the enzymes.

We chose to focus our studies on chitin synthase 7305 (chs7305, JGI-ID: 7305), because it is predicted to contain a myosin motor-like domain, which would indicate an intimate association of this chitin synthase with the actin cytoskeleton [18]. Actin has previously been found associated with the silica forming organelles of diatoms, the silica deposition vesicles (SDVs), and was hypothesized to influence silica biogenesis through yet unidentified transmembrane proteins in the SDV [4]. Furthermore, a chitin synthase from the mussel Mytilus galloprovincialis that also contains a predicted myosin motor domain was shown to be located in the developing shell, and was suggested to function in in the mineral biogenesis process [12].

Cultivation

T. pseudonana (CCMP1335) was grown in enriched artificial seawater medium according to the recipe of the North East Pacific Culture Collection [20] at 18 °C under constant light (4000–7000 lx).

Cloning and expression of recombinant proteins in T. pseudonana

The expression of chs7305 was done using the expression vector pTpNR/egfp which provides a switchable expression [21]. The chs7305 gene or gene fragments were amplified from genomic DNA with the oligonucleotides 5′-TTT GAT ATC ATG TCC TCT CGT CAC GAC GAC TC-3′ and 5′-ATA GGT ACC GCT CAT GCT ACG TTT GCT CCT CG-3′ (EcoRV and KpnI sites are underlined) to achieve a fusion upstream to egfp (C-terminal fusion protein). The PCR product was digested with EcoRV and KpnI and ligated into the vector pTpNR/EcoRV/KpnI/egfp. Furthermore, the oligonucleotides 5′-TTT GAT ATC ATG TCC TCT CGT CAC GAC GAC TC-3′, 5′-GCT TCT GCG TCT TTC TCG TCA GGG TAC CTT T-3′, 5′-TTT GCG GCC GCT TGG CTT CTT TGT GGG GAT CTT C-3′ and 5′-AAA GCG GCC GCT CAG CTC ATG CTA CGT TTG CTC-3′ (EcoRV, KpnI and NotI restriction sites are underlined) were used to obtain DNA fragments that split chs7305. The resulting fragments were ligated in the vector pTpNR/EcoRV/KpnI/egfp/NotI to insert egfp into chs7305 (the point of insertion locates in an extracellular domain of the corresponding protein sequence). The subsequent introduction of the expression vectors into T. pseudonana by particle bombardment and selection of recombinant cells on nourseothricin-containing agar plates was performed as described previously [21]. Successfully selected mutants were further analyzed by fluorescence microscopy and Western blotting.

Peptide antibody production and specificity tests

Peptide synthesis and subsequent immunization of rabbits was conducted by (Davids Biotechnologie (Regensburg, Germany). The peptide SEELQSTDKVCAQMTDEDKK was used as the target epitope region of chs7305. The antibody was affinity-purified by the manufacturer and the specificity was tested as follows. First, in a peptide competition assay (PCA), the synthesized peptide was pre-incubated at 10- and 100-times excess with anti-chs7305 for 1 h at 23 °C. The solution was then used for immunolocalization as described below. Second, the IgG fraction from pre-immune serum was isolated by G-Mag-Sepharose (GE Healthcare, Heidelberg, Germany) according to the manufacturer’s recommendations. This IgG fraction was subsequently used for the immunolocalization at the same protein concentration as anti-chs7305.

Immunofluorescence microscopy

Cells were harvested after 10 days of growth and the immunolabelling was carried out in 50 mM Tris-buffered saline (TBS, pH 7.5). After a single washing step, the cells were fixed in 2% formaldehyde for 2 h (23 °C, 0.1% Triton X-100). Subsequently, the cells were thoroughly washed and permeabilized in 1.5% Triton X-100 (1% BSA). The pellet was again thoroughly washed followed by a blocking step with a 1% BSA solution. The incubation with the primary antibody (anti-chs7305 peptide antibody) was carried out in a 1:50 dilution overnight at 4 °C. After thorough washing, anti-mouse IgG conjugated with CruzFluor488 (SantaCruz Biotechnology, Heidelberg, Germany) was applied in a 1:100 dilution. After incubation for 2 h at 23 °C, the sample was finally washed with TBS and analyzed by epifluorescence microscopy.

Immunofluorescently labeled cells were also stained with other fluorescent dyes. Calcofluor white was used to stain chitin in labeled cells. Those were incubated in a 0.01% solution (Tris–HCl, pH 8.8) for 10 min at room temperature after immunolocalization. PDMPO (2-(4-pyridyl)-5-((4-(2-dimethylaminoethyl-aminocarbamoyl)methoxy)-phenyl)oxazole) was used to stain newly formed frustules. Therefore, PDMPO was added to the growing culture 12 h prior to immunolocalization at a concentration of 10 µM.

Epifluorescence analysis was carried out with a LSM 780 laser scanning microscope (Zeiss, Göttingen, Germany) equipped with a laser diode (405 nm), Ar laser (488 nm) and HeNe laser (633 nm). The detection of fluorescence signals was achieved with a photomultiplier with adjustable band width. Fluorescence images were also recorded on an Axio Observer Z1 (Zeiss, Göttingen, Germany) equipped with a metal halide UV lamp and the filters FS 49: EX BP 347/55; BS LP 395; EM BP 445/50 (Dapi) FS 38 HE: EX BP 470/40; BS LP 495; EM BP 525/50 (GFP) and FS 50 HE: EX BP 640/30; BS LP 660; EM BP 690/50 (Cy5) for colocalization studies with calcofluor white and anti-chs7305.

Chitin staining with chitin-binding GFP (CB-GFP)

Chitin-binding GFP is a recombinant fusion protein of the chitin-binding domain of chitinase A from Paenibacillus sp. WL-12 (former Bacillus circulans WL-12) with green-fluorescent protein that specifically binds to chitin [12]. First, the staining conditions were tested at different pH values to determine interactions of CB-GFP (containing a His₆-tag) with silica. For this, calcined T. pseudonana cell walls were used. Biosilica was extracted as described previously [22] and subsequently calcined in a muffle furnace (Nabertherm) for 5 h at 550 °C which completely removes organic material from the cell walls [23].

The final chitin staining procedure started with an extraction with 100% methanol for 10 min at 23 °C. This reduced the intensive fluorescence of chloroplasts. Followed by thorough washing with 50 mM glycine–NaOH buffer (pH 10.0), a blocking step (1% BSA) for 1 h at 23 °C was conducted. The cell pellet was finally resuspended in an 80 ng/µL CB-GFP solution and incubated for 1 h at 23 °C. After three washing steps, fluorescence microscopy analysis was carried out.

Protein isolation/separation and western blotting

T. pseudonana was grown for 10 days and the culture was harvested for protein analysis. The cell pellets were washed with 50 mM Tris–HCl buffer (pH 7.0) and subsequently lysis buffer was applied (Tris–HCl, 2% SDS). After 30 min incubation at room temperature, the cell fragments were pelleted by centrifugation and the supernatant was kept for further analysis. Protein separation was then carried out by 10% SDS-Tris–glycine-PAGE. SDS-PAGE loading buffer (8 M urea, 100 mM Tris, 70 mM SDS) was added to the samples and a 5 min incubation at 37 °C was conducted. Following electrophoresis, proteins were transferred to an Amersham polyvinylidene fluoride (PVDF) membrane (GE Healthcare, Heidelberg, Germany) by electroblotting (Bio-Rad, Trans-Blot™ Cell) and an immunostaining was carried out in 50 mM TBS (pH 7.5). This started with an 8 h blocking step (5% milk powder, 0.05% Tween20, TBST milk), followed by the addition of anti-GFP antibody conjugated with horseradish peroxidase (SantaCruz Biotechnology, Heidelberg, Germany) at 1:1000 dilution in fresh TBST milk. Finally, the membrane was thoroughly washed with TBS. The luminescence reaction was conducted with SuperSignal WestPico (ThermoScientific; Rockford, USA) and detected on an Amersham X-Ray film (GE Healthcare, Heidelberg, Germany).

Initially chs7305 was expressed in T. pseudonana with the GFP gene fused to the C-terminus. However, the observed GFP localization pattern (Fig. 1a) appeared to indicate that the GFP is retarded in the endoplasmatic reticulum [26]. After gentle protein extraction to avoid membrane protein aggregation, Western blot analysis indicated that the expressed chs7305-GFP fusion protein was truncated and corresponds to the size of GFP itself (27 kDa) and not to the full-length fusion protein (159 kDa, Fig. 1b).

Localization experiments of chs7305. a Confocal fluorescence microscopy images of T. pseudonana transformants expressing the gene of the C-terminal chitin synthase 7305 fusion protein chs7305-CT-GFP and the corresponding Western blot results against GFP. The micrograph is an overlay of the recorded green channel (excitation: 488 nm, emission: 490–536 nm range) and the red channel (excitation: 633 nm, emission: 647–687 nm range). The green color represents GFP fluorescence, whereas the red color is caused by chloroplast autofluorescence. b Western blot analysis (against GFP) of T. pseudonana transformants expressing the gene of the chitin synthase 7305 fusion protein chs7305-ED-GFP (159 kDa) with the GFP gene within the extracellular domain E1. c Schematic representation of the domain structure of chs7305 (132 kDa) and the locations of recombinant GFP introduction (green arrows). C: cytosolic domain, E: extracellular domain, TM: transmembrane domain

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The position of GFP was then switched to an extracellular domain of chs7305, which led to no fluorescence at all. Surprisingly, GFP was still detectable by Western blot analysis. However, again the size of the resulting GFP fusion protein was considerably smaller (~ 38 kDa) than the predicted size (159 kDa). This result was confirmed by the investigation of at least three independent positive egfp-containing clones. The mechanism which lead to the small protein size observed after Western blotting is unclear. The reasons for the absence of GFP fluorescence and the detection of only partial fusion proteins were not investigated further and remain elusive. However, a possible cause for this might be the quenching of GFP fluorescence by acidic conditions inside a vesicle.

The small fusion protein size and the localization pattern raised concerns about the applicability of this approach for the localization of chitin synthases in T. pseudonana. Consequently, we decided to pursue immunolocalization. Polyclonal antibodies were raised against four synthetic peptides specific for the T. pseudonana chitin synthases: chs7305, chs6575, chs4368 and chs4413. Since only the antibodies against chs7305 showed a specific signal with respect to the control experiments (see experimental section), the chitin synthase chs7305 was chosen for the final study. Immunolocalization with anti-chs7305 resulted in well-defined fluorescence patterns (Fig. 2). In all cell cycle stages the immunostained cells exhibited a pattern of regularly spaced fluorescent dots at the rim of the valve region (Fig. 2a, b). Cells that were close to cell division (i.e. elongated cells) exhibited an additional fluorescent ring along the entire central region of the cell wall (Fig. 2a).

Images obtained by confocal immunofluorescence microscopy of T. pseudonana. Samples were prepared by immunlocalization of chs7305 in wild type cells using (a) anti-chs7305. b IgG fraction isolated from preimmune serum, and c anti-chs-7305 preincubated with 100-times excess of peptide. Each micrograph is an overlay of two images of the recorded green channel and the red channel (settings according to Fig. 1). The green color represents CFL488 fluorescence (secondary antibody), the red color is caused by chloroplast autofluorescence. The scale bar is valid for images b and c

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Subsequently, a peptide competition assay (PCA) and immunolocalization with the isolated IgG fraction of the preimmune serum were conducted to investigate the specificity of the peptide antibody. The continuous central ring was absent when isolated IgGs from preimmune serum were used, whereas the dot pattern remained unchanged (Fig. 2b). This was in agreement with PCA using a 100-times molar excess of peptide vs. antibody, which resulted in absence of the ring while the dots were still visible. These results revealed that only the the ring is a specific signal and represents the location of chs7305.

To investigate the location of chs7305 relative to the biosilica-associated chitin, immunolabelling with anti-chs7305 antibodies was followed by calcofluor white staining to visualize the chitin. Figure 3 shows that chs7305 and chitin are almost perfectly co-localized as ring-shaped structures in the mid region of the cell wall. As an alternative probe for chitin, CB-GFP was used for the co-localization experiment. CB-GFP is a green fluorescent protein that carries a chitin binding (CB) domain and has previously been used to localize chitin in mollusc shells [12, 24]. The CB-GFP staining confirmed the results obtained with calcofluor white (not shown).

Confocal fluorescence microscopy of immunofluorescently labeled cells of T. pseudonana (anti-chs7305). The colocalization of chs7305 with chitin by calcofluor white is shown. Beside the bright field images (left side), fluorescence channels are shown as follows: calcofluor white (excitation: UV, emission: BP 445/50 filter) and anti-chs7305 (excitation: UV, emission: BP 525/50). The fluorescence channels were merged as depicted right. Red fluorescence originates from chloroplast autofluorescence (detected as separate channel)

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These results strongly suggest that chs7305 is responsible for the synthesis of the chitin-based ring that is present in the mid-cell region. However, this observation was limited to cell populations that were grown for longer time periods (≥ 10 days). Under these conditions nutrients become limited. During the early phase of growth under abundant nutrient conditions, elongated cells neither showed the presence of chs7305 nor of the chitin-based ring structure (not shown). This observation agrees with the extremely low transcript abundance of chs7305 and the chitin-binding protein genes p150 and p150-like. It indicates that chitin synthesis, in context of the chitin-based ring, is predominately relevant when nutrients become scarce. This suggests that the production of chs7305 and the chitin-based ring could be an adaptation to nutrient limitation. Furthermore, the localization pattern of a girdle band-associated protein, p150, fits well with the localization observed in this study. p150 is highly upregulated under stress conditions such as high copper and low silicon or iron concentrations [25].

To investigate potential functional connections between chs7305, p150, and p150-like their mRNA abundance in dependence on the cell density was compared (Fig. 4). This clearly shows that the three genes were drastically upregulated in the late growth phase. Compared to the exponential growth phase (0.5*10⁶ cells/mL), chs7305, p150, and p150-like are 13-, 234-, and 25-times upregulated in the stationary phase (2.0*10⁶ cells/mL).

Transcript abundance of chitin synthase 7305 and the chitin-binding proteins p150 and p150-like. The abundance is given as reads per kilobase per million mapped reads (RPKM)

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The occurrence and the localization pattern of chs7305 and chitin also fits well with localization studies previously conducted with T. pseudonana and other diatom species [18]. The authors of this study detected chitin in silicic acid-starved cells of several diatom species and interpreted its appearance as an adaptation of frustule formation under changing environmental conditions. This suggests that chitin could be an important component in the adaptation to the reduction of nutrients. The depletion of silicic acid from the growth medium may require stabilizing support for the silica-based cell walls. A chitin-based structure could be able to provide additional strength to the cells walls so that its integrity can be preserved. This stabilization is, in turn, not required during early growth stages where sufficient silicic acid is available to form more stable cells walls. This is supported by transcriptome and proteome analyses which also detected an increased expression of chitin-related genes under different nutrient limitations [26,27,28,29] and is in agreement with the observation that chs7305 is detectable in cultures grown for longer time periods, when the nutrient concentration is significantly decreased.

Chitin-based ring structures are also known from other organisms. For instance, budding yeasts produce a primary septum composed of chitin during cell division suggesting an involvement of the chitin synthase in separation of the mother and daughter cell [30, 31]. Degradation of the primary septum by a chitinase enables the mother and daughter cell to separate [32]. Chitin-binding proteins, such as p150, could induce the controlled degradation of the observed chitin-based ring. It is known that chitinolytic enzymes such as chitin-active lytic polysaccharide monooxygenases bind to chitin and in some cases produce nicks by an oxidative reaction [33]. Thus, chs7350 and p150 could be part of a regulative machinery that controls cell wall integrity in the girdle band region. This may give an explanation of the observation of elongated cell morphologies in course of the upregulation of p150.

The investigations on chs7305 from T. pseudonana showed that this chitin synthase is not involved in the formation of chitin fibers, but in the formation of a chitin-based ring at the girdle band region of elongated cells after growth for 10 days or longer. Interestingly, the chitin meshwork found in T. pseudonana was also isolated under similar condition. This indicates that the chitin-based ring might play a role for stabilization of the cell wall. It will be of interest to see, whether similar chitin structures can also be found in other diatoms harboring several potential chitin synthase genes. For experimental elucidation of the function of the chitin-based ring structure, knock-out or knock-down experiments will be necessary.

All data generated or analyzed during this study are included in the article. Data sets from individual experiments can be obtained from the corresponding authors upon reasonable request.

BSA:

bovine serum albumin

CB-GFP:

chitin-binding green-fluorescent protein

CT:

carboxy terminal

GFP:

green-fluorescent protein

IgG:

immunglobulin G

kDa:

kilo Dalton

LCPA:

long chain polyamines

PAGE:

polyacrylamide gel electrophoresis

PCA:

peptide competition assay

PDMPO:

(2-(4-pyridyl)-5-((4-(2-dimethylaminoethyl-aminocarbamoyl)methoxy)-phenyl)oxazole)

PVDF:

polyvinylidene fluoride

RPKM:

reads per kilobase per million mapped reads

SDS:

sodium dodecyl sulfate

Tris:

tris(hydroxymethyl)aminomethane

UV:

ultraviolet

The authors thank the Deutsche Forschungsgemeinschaft for financial support through Research Unit 2038 “NANOMEE” (PE 348/31-1 and KR 1853/8-2) The calcination of biosilica by C. Fischer (TU Dresden) is gratefully acknowledged. We would like to thank Ingrid Weiss (University Stuttgart) for kindly providing the CB-GFP plasmid, and Beate Brankatschk (TU Dresden) for technical support.

This research was funded by the Deutsche Forschungsgemeinschaft (PE 348/31-1 and KR 1853/8-2). The funding body played no roles in the design of the study and collection, analysis, and interpretation of data and in writing the manuscript.

Authors and Affiliations

1. General Biochemistry, Technical University of Dresden, 01062, Dresden, Germany

   Martin Wustmann & Karl-Heinz van Pée

2. B CUBE – Center for Molecular Bioengineering, Technical University of Dresden, Tatzberg 41, 01307, Dresden, Germany

   Nicole Poulsen & Nils Kröger

3. Cluster of Excellence Physics of Life, TU Dresden, 01062, Dresden, Germany

   Nils Kröger

4. Faculty of Chemistry and Food Chemistry, TU Dresden, 01062, Dresden, Germany

   Nils Kröger

Contributions

MW planned and performed the experiments and wrote the manuscript. NP was involved in the planning of some of the experiments and in writing the manuscript. NK contributed to the writing of the manuscript. K-HvP designed and supervised the study and contributed to the writing of the manuscript. All authors have read and approved the manuscript.

Corresponding author

Correspondence to Karl-Heinz van Pée.

Competing interests

The authors declare that they have no competing interests.

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