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Plant Physiol, September 2001, Vol. 127, pp. 8-9
THE HOT AND THE CLASSIC
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INTRODUCTION |
A novel reproductive feature of the
seed plants that enabled them to colonize drier regions of the
terrestrial environment was the pollen tube, a structure that serves to
deliver sperm to the egg and central cell of the
megagametophyte. Pollen, however, is not deposited directly on
the megagametophyte that would be too easy. Each pollen grain must
prove its mettle to the female, first by landing successfully
on the stigmatic surface, then by germinating, and finally
by elongating across the entire length of the long style. Three of the
more interesting physiological questions surrounding this
process include: how do pollen tubes achieve their phenomenal rates of
growth, how do pollen tubes sense the location of the megagametophyte,
and how do self-incompatibility reactions effectively remove some of
the pollen grains from the race to the egg? This week's The Hot
and the Classic summarizes 11 of the more highly cited pollen tube
papers of the 1990s that bear upon these questions.
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Calcium Channels Needed for Pollen Tube
Elongation |
Pierson et al. (1994) provide a detailed spatial analysis of the
steep Ca2+ gradient that exists in the tips of
pollen tubes. They confirm that the high
[Ca2+]cyt at the tip
arises from a highly localized influx of Ca2+
ions. Injection of intracellular Ca2+ buffers or
application of elevated levels of Suc reversibly inhibits growth,
destroys tip zonation of organelles, and modifies normal patterns of
cytoplasmic streaming. These treatments also dissipate both the
intracellular tip-focused gradient and the extracellular Ca2+ flux. These findings provide evidence that
growing pollen tubes have open Ca2+ channels in
their tip and that these channels become inactivated in non-growing tubes.
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Phosphoinositide Turnover and Pollen Tube Growth |
Franklin-Tong et al. (1996) demonstrate that the
pollen tubes of Papaver rhoeas have a
Ca2+-dependent polyphosphoinositide-specific
phospholipase C (PLC) activity that is inhibited by neomycin. The
photolysis of caged inositol (1,4,5)-trisphosphate
(IP3) in pollen tubes reveals that IP3 induces an intracellular release of
Ca2+ ions, which is inhibited by heparin and
neomycin. Mastoparan, which stimulates IP3
production, also induces a rapid neomycin-sensitive increase in
[Ca2+]cyt. These data
provide direct evidence for the involvement of a functional
phosphoinositide signal-transducing system in pollen tubes.
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Cytoplasmic Ca2+ Controls the Axis
of Pollen Tube Growth |
Malho and Trewavas (1996) report that increasing
[Ca2+]cyt on one side of
the pollen tube apex induces reorientation of the growth axis toward
that side. Similarly, a decrease in
[Ca2+]cyt promoted
bending toward the opposite side. These effects are mimicked by
imposing localized external gradients of an ionophore (A23187) or a
Ca2+ channel blocker (GdCl3); the pollen tubes
bend toward the highest concentration of A23187 and away from
GdCl3. Manipulation of [Ca2+]cyt
in regions farther back from the apical zone also induces changes
in growth direction, but the new orientation is random.
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Calcium Oscillations |
Pierson et al. (1996) report that a steep tip-focused gradient
occurs in the elongating pollen tubes of all species examined. Analysis
of Lilium longiflorum pollen tubes loaded with
dextran-conjugated fura-2 reveals that the gradient derives from
Ca2+ entry that is restricted to a small area of
plasma membrane at the extreme apex of the tube dome. The authors
propose that since the apical membrane is continually swept to the
shanks during tube elongation, either Ca2+
channels are specifically retained at the extreme apex or the Ca2+ channels at the tip rapidly inactivate as
new ones are inserted during vesicle fusion. The peak of the
[Ca2+]cyt gradient
fluctuates in magnitude from 0.75 to above 3 µM, with the elevated points being
correlated with an increased rate of tube growth (see also
Franklin-Tong, 1996; Mahlo and Trewavas, 1996; Holdaway-Clarke et al.,
1997). Inhibition of pollen tube growth caused by various
treatments is correlated with the dissipation of both the
tip-focused gradient and the Ca2+ influx.
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G-Proteins Regulate Pollen Tube Elongation |
Pollen tube elongation depends on actin-dependent targeted
secretion at the tip. Because small GTPases of the Rho family, which
are homologs of Rac and Cdc42, have been implicated in the regulation
of related processes in animal and yeast cells, two recent studies
examined the possible role of Rho-type G-proteins in pollen tube
elongation (Kost et al., 1999; Li et al., 1999).
Kost et al. (1999) demonstrated that the expression of a
non-functional mutant Rho-type G-protein in Arabidopsis inhibited pollen tube elongation, whereas expression of a constitutively active
Rho-type G-protein caused depolarized growth (see also Li et al.,
1999). Rho-type G-protein was found to accumulate at the pollen tube
tip plasma membrane and to be physically associated with
phosphatidylinositol monophosphate kinase (PI P-K) and its product,
phosphatidylinositol 4,5 bisphosphate (PtdIns
4,5-P2). The expression of a PLC domain that
binds specifically to PtdIns 4,5-P2 also
inhibited pollen tube elongation. The authors propose that Rho-type
G-proteins may control the local activity of PI P-K in the tip of the
pollen tube and that the product of PI P-K, PtdIns
4,5-P2, may serve as a substrate for the
production of IP3 by PLC.
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Gametophytic Self-Incompatability |
Gametophytic self-incompatibility provides a
genetic barrier to self-fertilization, and in the simplest cases is
controlled by the highly polymorphic S locus. Growth of a pollen tube
in the style is arrested when the S allele carried by the pollen matches either one of the two S alleles carried by the pistil. Putative
S allele proteins of the pistil, which are RNases, had been shown to
co-segregate with S alleles, but there had been only correlative or
indirect evidence for the claim that these S allele-associated
proteins (S proteins) are involved in recognition and
rejection of self-pollen. The study of Lee et al. (1994) demonstrated that the inhibition of synthesis of S2 and S3 proteins in Petunia inflata plants of S2S3 genotype by the antisense S3 gene resulted in failure of the transgenic plants to reject S3 and S2
pollen. The expression of the transgene encoding S3 protein
in P. inflata plants of S1S2 genotype confers on the
transgenic plants the ability to reject S3 pollen (see also Murfett et
al., 1994). These findings provide direct in vivo evidence that S
proteins control the self-incompatibility behavior of the pistil.
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A Stylar Glycoprotein Aids Pollen Tube Growth |
When compared to pollen tubes that grow naturally
(i.e. through stylar tissue), pollen tubes grown in vitro extend in
random directions, exhibit reduced growth rates, and grow to shorter final lengths. Since pollen tubes elongate through the extracellular matrix of the stigma and the style, it has been proposed that the
extracellular matrix of the pistil provides chemical and physical support as well as directional cues for the elongating pollen tube.
Cheung et al. (1995) purified a glycoprotein, TTS, from tobacco
(Nicotiana alata) stylar transmitting tissue, that supports pollen tube growth between the stigma and the ovary. TTS proteins belong to the arabinogalactan protein family, stimulate
pollen tube growth in vitro, and attract pollen tubes grown in a
semi-in vivo culture system. In vivo, the pollen tube growth rate is
reduced in transgenic plants that have significantly reduced levels of TTS proteins as a result of either anti-sense suppression or sense co-suppression. These results identify the TTS protein as a pistil component that facilitates pollen tube growth.
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Lipids Regulate Pollen Penetration of
Papillae |
Pollen hydration, germination, and penetration of the stigma by
pollen tubes are influenced by the exudate on wet stigmas. Wolters-Arts
et al. (1998) tested selected compounds for their ability to act as
functional substitutes for exudate in the initial stages of pollen-tube
growth on transgenic stigmaless tobacco plants that did not produce
exudate. They found that lipids are the essential factor needed for
pollen tubes to penetrate the stigma and that, in the presence of these
lipids, pollen tubes will also penetrate leaves. They propose that
lipids direct pollen-tube growth by controlling the flow of water to
pollen in species with wet stigmas.
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LITERATURE CITED |
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Cheung AY, Wang H, Wu HM
(1995)
A floral transmitting tissue-specific glycoprotein attracts pollen tubes and stimulates their growth.
Cell
82: 383-393[CrossRef][Web of Science][Medline]
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Franklin-Tong VE, Drobak BK, Allan AC, Watkins PAC, Trewavas AJ
(1996)
Growth of pollen tubes of Papaver rhoeas is regulated by a slow-moving calcium wave propagated by inositol 1,4,5-trisphosphate.
Plant Cell
8: 1305-1321[Abstract]
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Holdaway-Clarke TL, Feijo JA, Hackett GR, Kunkel JG, Hepler PK
(1997)
Pollen tube growth and the intracellular cytosolic calcium gradient oscillate in phase while extracellular calcium influx is delayed.
Plant Cell
9: 1999-2010[Abstract]
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Kost B, Lemichez E, Spielhofer P, Hong Y, Tolias K, Carpenter C, Chua NH
(1999)
Rac homologues and compartmentalized phosphatidylinositol 4,5-bisphosphate act in a common pathway to regulate polar pollen tube growth.
J Cell Biol
145: 317-330[Abstract/Free Full Text]
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Lee HS, Huang SS, Kao TH
(1994)
S-Proteins control rejection of incompatible pollen in Petunia inflata.
Nature
367: 560-563[CrossRef][Medline]
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Li H, Lin YK, Heath RM, Zhu MX, Yang Z
(1999)
Control of pollen tube tip growth by a pop GTPase-dependent pathway that leads to tip-localized calcium influx.
Plant Cell
11: 1731-1742[Abstract/Free Full Text]
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Malho R, Trewavas AJ
(1996)
Localized apical increases of cytosolic free calcium control pollen tube orientation.
Plant Cell
8: 1935-1949[Abstract]
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Murfett J, Atherton AL, Mou B, Gasser CS, McClure BA
(1994)
S-RNase expressed in transgenic Nicotiana causes S-allele-specific pollen rejection.
Nature
367: 563-566[CrossRef][Medline]
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Pierson ES, Miller DD, Callaham DA, Shipley AM, Rivers BA, Cresti M, Hepler PK
(1994)
Pollen-tube growth is coupled to the extracellular calcium-ion flux and the intracellular calcium gradient: effect of BAPTA-type buffers and hypertonic media.
Plant Cell
6: 1815-1828[Abstract/Free Full Text]
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Pierson ES, Miller DD, Callaham DA, van Aken J, Hackett G, Hepler PK
(1996)
Tip-localized calcium entry fluctuates during pollen tube growth.
Dev Biol
174: 160-173[CrossRef][Web of Science][Medline]
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Wolters-Arts M, Lush WM, Mariani C
(1998)
Lipids are required for directional pollen-tube growth.
Nature
392: 818-821[CrossRef][Medline]
Peter V. Minorsky
Department of Biology
Vassar College
Poughkeepsie, NY 12604
© 2001 American Society of Plant Physiologists
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INTRODUCTION
Calcium Channels Needed for...