Copyright ©The Histochemical Society, Inc.

BRIEF REPORT

Uptake of a Fluorescent Dye as a Swift and Simple Indicator of Organelle Intactness : Import-competent Chloroplasts from Soil-grown Arabidopsis

Alexander Schulz, Jürgen Knoetzel, Henrik V. Scheller and Alexandra Mant

Plant Biochemistry Laboratory (JK,HVS,AM) and Plant Anatomy and Physiology Laboratory (AS), The Royal Veterinary and Agricultural University, Copenhagen, Denmark

Correspondence to: Alexandra Mant, Plant Biochemistry Laboratory, The Royal Veterinary & Agricultural University, 40, Thorvaldsensvej, DK-1871 Frederiksberg C, Copenhagen, Denmark. E-mail: ama{at}kvl.dk


    Summary
 Top
 Summary
 Literature Cited
 
We developed a rapid and reliable technique for specifically staining intact chloroplasts using the fluorescent dye carboxyfluorescein diacetate. Intact, import-competent chloroplasts were isolated simply and rapidly from soil-grown Arabidopsis thaliana plants, with yields of 20 ± 5 µg chlorophyll per g FW, greater than previously reported yields from soil-grown Arabidopsis. Traditional chloroplast isolation buffers sometimes contain low concentrations (<10 mM) sodium ascorbate as a general-purpose anti-oxidant, but we found that only Arabidopsis chloroplasts isolated in the presence of high concentrations (50–100 mM) of sodium ascorbate in the initial grinding buffer were import-competent. (J Histochem Cytochem 52:701–704, 2004)

Key Words: carboxyfluorescein diacetate • intact organelles • Arabidopsis • chloroplast • glucosinolates • protein import

UNDERSTANDING organelle biogenesis relies on the isolation of intact organelles for characterization of import and targeting of nuclear-encoded precursor proteins. Much attention has focused on the biogenesis of chloroplasts. Although these organelles are plant-specific, their protein targeting machinery shares features in common with ER, mitochondria, and the prokaryotic plasma membrane, and they provide an excellent model system in which to study protein-membrane interactions. Indeed, the TAT (twin-arginine translocase) export system was identified first in thylakoids and then in the E. coli plasma membrane. Few species yield import-competent chloroplasts, so most work has exploited pea as a model system. The complete sequencing of the Arabidopsis genome and the ease with which this plant can be manipulated genetically enable us to identify and create useful mutants with altered or missing components of the protein translocation machinery. Progress with Arabidopsis has been hampered by low yields of intact chloroplasts, relatively inefficient protein uptake, and a high degree of nonspecific binding of precursor proteins to the outside of the organelles. These issues have been addressed recently in two studies, the first of which described isolation of chloroplasts from protoplasts (Fitzpatrick and Keegstra 2001Go) and the second homogenization of entire seedlings (Aronsson and Jarvis 2002Go). However, both methods use seedlings grown on sterile medium, which is laborious. We report improved import efficiency of intact chloroplasts isolated from soil-grown Arabidopsis. This rapid method is useful because active chloroplasts can be isolated from batches of plant material used for parallel types of study, e.g., measurements of photosynthetic activity.

Arabidopsis thaliana ecotype Columbia was grown on compost under low light (100 µmol photon m–2 sec–1) with an 8-hr photoperiod at 20 ± 2C for 4–5 weeks. Chloroplasts were isolated using a linear Percoll gradient essentially according to the barley method described in Brock et al. (1993)Go with the following modifications: 10 g healthy leaves were homogenized in 200 ± 50 ml grinding buffer containing 50 mM L (+) sodium ascorbate, in four 2-sec pulses in a kitchen blender equipped with disposable razor blades (Kannangara et al. 1977Go), and all centrifugation except the Percoll gradient step was reduced to 1000 x g. Larger quantities of leaf material (20–40 g tissue) required 100 mM sodium ascorbate in the initial grinding buffer. Typical yields were 20 ± 5 µg chlorophyll per g FW, which are greater than published yields from similar tissue [5 µg/g FW (Fitzpatrick and Keegstra 2001Go); 4–6 µg/g FW (Rensink et al. 1998Go)]. Traditional grinding buffers have sometimes included 1–10 mM sodium ascorbate or isoascorbate as a general-purpose anti-oxidant (e.g., Walker et al. 1987Go). We propose an additional role for sodium ascorbate in protecting Arabidopsis chloroplasts from damage by the breakdown products of glucosinolates. Glucosinolates are abundant in Arabidopsis; tissue damage leads to their hydrolysis by myrosinases (Wittstock and Halkier 2002Go). It is well documented that glucosinolate breakdown products are biologically active and can cause enzyme and organelle damage (e.g., Lykkesfeldt and Møller 1993Go). L-Ascorbic acid is a specific inhibitor of myrosinases when used at 50–100 mM but activates myrosinases at 0.1–10 mM (Ohtsuru and Hata 1973Go). Therefore, it is important to use ascorbate at concentrations >=50 mM.

Chloroplast intactness, necessary for protein import assays, is often estimated by phase-contrast microscopy (Walker et al. 1987Go). Intact chloroplasts are surrounded by a more pronounced halo (Figures 1A and 1C) compared with broken chloroplasts (Figure 1B). One drawback with this method is that chloroplast envelopes can break, releasing stromal contents, and then reseal, retaining the appearance of intactness (Walker et al. 1987Go). Arabidopsis chloroplasts were equilibrated for 5 min with an equal volume of carboxyfluorescein diacetate (CFDA; Molecular Probes, Leiden, The Netherlands), final concentration 0.0025% w/v, and were examined with a Zeiss Photomikroskop II equipped with FITC filters (excitation filter BP 455–490, beam splitter FT 510, and emission filter, either "fluorescein-specific" BP 520–560 or "nonspecific" LP 520). CFDA fluoresces strongly when de-esterified to carboxyfluorescein (CF). "Ester loading" of nonpolar esterified derivatives of fluorescein is a standard test for cell viability, depending on an intact membrane that prevents leakage of the polar dye into the medium and on the presence of esterases (Oparka and Read 1994Go). Chloroplasts that had taken up CFDA fluoresced intensely green (Figure 1E) and corresponded exactly to the ones delineated by a bright halo under phase-contrast (Figure 1D). Up to three Arabidopsis carboxylesterases are predicted to be targeted to the chloroplast stroma (Swissprot Q9M899, Q8L8W1, Q9LT10; Emanuelsson et al. 2000Go), implying that the green-fluorescing organelles retain stromal contents as well as an intact envelope. Interestingly, the non-carboxylated dye fluorescein diacetate did not cause fluorescence of chloroplasts (data not shown). Chloroplasts that did not take up CFDA (Figures 1D–1F, marked with arrows) were red when all emission wavelengths (F) or only chlorophyll autofluorescence (not shown) were detected using appropriate filters. Red chloroplasts corresponded exactly to the ones without a marked halo under phase-contrast. With the nonspecific filter settings, intact chloroplasts appeared yellowish owing to the presence of both green fluorescein and red autofluorescence. Chloroplasts isolated in the absence of ascorbate (Figures 1G–1I) were not visibly damaged and showed a similar degree of intactness as those isolated in the presence of ascorbate (Figures 1D–1F).



View larger version (75K):
[in this window]
[in a new window]
 
Figure 1

Images of isolated Arabidopsis and pea chloroplasts analyzed by brightfield, phase-contrast, and fluorescence microscopy. (A) Arabidopsis chloroplasts isolated in the presence of sodium ascorbate, phase-contrast objective. (B) Broken Arabidopsis chloroplasts recovered from the "lysed" fraction of the Percoll gradient, phase-contrast objective. (C) Pea chloroplasts isolated by standard procedures without sodium ascorbate, phase-contrast objective. (D–F) Arabidopsis chloroplasts isolated in the presence of sodium ascorbate and incubated with CFDA, viewed with brightfield objective (D), fluorescein-specific filter (E), and nonspecific wavelengths filter to monitor CFDA and chlorophyll fluorescence (F). (G–I) Arabidopsis chloroplasts isolated without sodium ascorbate and incubated with CFDA, viewed with phase-contrast objective (G), fluorescein-specific filter (H), and nonspecific wavelengths filter (I). Bars = 10 µm. Arrows point to broken chloroplasts.

 
There was, however, a marked difference in the chloroplasts' ability to import precursor proteins (Figure 2) . Import assays were carried out according to Robinson and Mant (2002)Go using the pea precursor of Rubisco small subunit (pSSU, a stromal protein), and the wheat precursor of the 33-kD oxygen-evolving complex subunit (p33K, a thylakoid lumen protein). Chloroplasts were fractionated after import to determine the location of imported protein. For chloroplasts isolated without ascorbate, the majority of chloroplast-associated radiolabeled protein was precursor, bound to the outside of the organelle (Figure 2A, no ascorbate). Little SSU was found in the stromal fraction, and almost no 33K in the thylakoid lumen. By contrast, for chloroplasts isolated in the presence of 50 mM ascorbate (Figure 2A, with ascorbate), the majority of radiolabeled protein was protected from protease digestion and correctly targeted to the stromal and thylakoid lumen compartments, respectively. A parallel experiment using pea chloroplasts isolated by standard procedures without ascorbate (Figure 1C) showed that Arabidopsis import efficiencies were on a par with those of pea (Figure 2B).



View larger version (45K):
[in this window]
[in a new window]
 
Figure 2

Comparison of the protein import capabilities of chloroplasts isolated in the presence and absence of sodium ascorbate. (A) Arabidopsis chloroplasts isolated in the absence (– Ascorbate) or presence (+ 50 mM Ascorbate) were incubated with radiolabeled precursor proteins, fractionated, and analyzed by SDS-PAGE and fluorography. Tr, in vitro translation mixture; C, total washed chloroplasts; C+, protease-treated chloroplasts; S, stromal extract; T, total membranes (mainly thylakoids with some envelopes); T+, protease-treated membranes; Tr+, protease-treated in vitro translation mixture. (B) Pea chloroplasts isolated in the absence of sodium ascorbate, gel lanes as in A. (C) Comparison of rate of protein import for Arabidopsis chloroplasts isolated in the presence of 0, 10, and 50 mM ascorbate.

 
We compared the rate of pSSU import by Arabidopsis chloroplasts isolated in the absence of ascorbate and in the presence of 10 mM and 50 mM ascorbate (Figure 2C). Chloroplasts isolated in the presence of 50 mM ascorbate imported pSSU at a rate 19-fold and 11-fold higher than in the absence of ascorbate or presence of 10 mM ascorbate, respectively.

We conclude that inclusion of 50 mM ascorbate in the grinding buffer enables the isolation of import-competent chloroplasts. The use of CFDA to identify intact chloroplasts may also be extended to other isolated organelles containing carboxylesterases.


    Acknowledgments
 
Supported by an EMBO Long Term Fellowship to AM.

We thank Mitsuru Akita and Kenneth Keegstra for giving the clone encoding pea pSSU, Birger L. Møller for invaluable advice and Lynda Fitzpatrick for helpful discussions.


    Footnotes
 
Received for publication January 12, 2004; accepted January 14, 2004


    Literature Cited
 Top
 Summary
 Literature Cited
 

Aronsson H, Jarvis P (2002) A simple method for isolating import-competent Arabidopsis chloroplasts. FEBS Lett 529:215–220[Medline]

Brock IW, Hazell L, Michl D, Nielsen VS, Møller BL, Herrmann RG, Klösgen RB, et al. (1993) Precursors of one integral and five luminal thylakoid proteins are imported by isolated pea and barley thylakoids: optimisation of in vitro assays. Plant Mol Biol 23:717–725[Medline]

Emanuelsson O, Nielsen H, Brunak S, von Heijne G (2000) Predicting subcellular localization of proteins based on their N-terminal amino acid sequence. J Mol Biol 300:1005–1016[Medline]

Fitzpatrick LM, Keegstra K (2001) A method for isolating a high yield of Arabidopsis chloroplasts capable of efficient import of precursor proteins. Plant J 27:59–65[Medline]

Kannangara CG, Gough SP, Hansen J, Rasmussen N, Simpson DJ (1977) A homogenizer with replaceable razor blades for bulk isolation of active barley plastids. Carlberg Res Commun 42:431–439

Lykkesfeldt J, Møller BL (1993) Synthesis of benzylglucosinolate in Tropaeolum majus—L-isothiocyanates as potent enzyme-inhibitors. Plant Physiol 102:609–613[Abstract/Free Full Text]

Ohtsuru M, Hata T (1973) Studies on the activation mechanism of the myrosinase by L-ascorbic acid. Agr Biol Chem 37:1971–1972

Oparka KJ, Read ND (1994) The use of fluorescent probes for studies on living plant cells. In Harris N, Oparka, KJ, eds. Plant Cell Biology—A Practical Approach. Oxford, Oxford University Press, 27–50

Rensink WA, Pilon M, Weisbeek P (1998) Domains of a transit sequence required for in vivo import in Arabidopsis chloroplasts. Plant Physiol. 118:691–699[Abstract/Free Full Text]

Robinson C, Mant A (2002) Import of proteins into isolated chloroplasts and thylakoid membranes. In Gilmartin P, Bowler C, eds. Molecular Plant Biology. Vol 2. A Practical Approach. Oxford, Oxford University Press, 123–146

Walker DA, Cerovic ZG, Robinson S (1987) Isolation of intact chloroplasts: general principles and criteria of integrity. Methods Enzymol 148:145–157

Wittstock U, Halkier BA (2002) Glucosinolate research in the Arabidopsis era. Trends Plant Sci 7:263–270[Medline]