Chlorophyll fluorescence

{{main|Kautsky effect}}

Upon illumination of a dark-adapted leaf, there is a rapid rise in fluorescence from Photosystem II (PSII), followed by a slow decline. First observed by Kautsky et al., 1932, this is called the Kautsky Effect. This variable rise in chlorophyll fluorescence is due to photosystem II.{{cite journal | last1 = Zhu | first1 = X-G. | last2 = Govindjee | first2 = Baker N.R. | last3 = Ort | first3 = D.R. | last4 = Long | first4 = S.P. | year = 2005 | title = Chlorophyll a fluorescence induction kinetics in leaves predicted from a model describing each discrete step of excitation energy and electron transfer associated with Photosystem II | journal = Planta | volume = 223 | issue = 1| pages = 114–133 | doi = 10.1007/s00425-005-0064-4 | pmid = 16411287 | bibcode = 2005Plant.223..114Z | s2cid = 9698923 }} Fluorescence from photosystem I is not variable, but constant.

The increase in fluorescence is due to PSII reaction centers being in a "closed" or chemically reduced state.{{cite journal | last1 = Zhu | first1 = X-G. | last2 = Govindjee | last3 = Baker | first3 = N.R. | last4 = de Sturler | first4 = E. | last5 = Ort | first5 = D.R. | last6 = Long | first6 = S.P. | year = 2005 | title = Chlorophyll a fluorescence induction kinetics in leaves predicted from a model describing each discrete step of excitation energy and electron transfer associated with Photosystem II | url = http://www.math.vt.edu/people/sturler/publications/Planta_FluorescenceInSilico_FinalSubmission_20050310.pdf | journal = Planta | volume = 223 | issue = 1| pages = 114–133 | doi = 10.1007/s00425-005-0064-4 | pmid = 16411287 | bibcode = 2005Plant.223..114Z | s2cid = 9698923 }} Reaction centers are "closed" when unable to accept further electrons. This occurs when electron acceptors downstream of PSII have not yet passed their electrons to a subsequent electron carrier, so are unable to accept another electron. Closed reaction centres reduce the overall photochemical efficiency, and so increases the level of fluorescence. Transferring a leaf from dark into light increases the proportion of closed PSII reaction centres, so fluorescence levels increase for 1–2 seconds. Subsequently, fluorescence decreases over a few minutes. This is due to; 1. more "photochemical quenching" in which electrons are transported away from PSII due to enzymes involved in carbon fixation; and 2. more "non-photochemical quenching" in which more energy is converted to heat.

Usually the initial measurement is the minimal level of fluorescence, $\backslash ,F\_0$. This is the fluorescence in the absence of photosynthetic light.

To use measurements of chlorophyll fluorescence to analyse photosynthesis, researchers must distinguish between photochemical quenching and non-photochemical quenching (heat dissipation). This is achieved by stopping photochemistry, which allows researchers to measure fluorescence in the presence of non-photochemical quenching alone. To reduce photochemical quenching to negligible levels, a high intensity, short flash of light is applied to the leaf. This transiently closes all PSII reaction centres, which prevents energy of PSII being passed to downstream electron carriers. Non-photochemical quenching will not be affected if the flash is short. During the flash, the fluorescence reaches the level reached in the absence of any photochemical quenching, known as maximum fluorescence $\backslash ,F\_m$.{{cite web |url=http://jxb.oxfordjournals.org/content/51/345/659.full.pdf+html |title=Chlorophyll fluorescence—a practical guide |publisher=Jxb.oxfordjournals.org |date=2000-04-01 |access-date=2011-03-28 |archive-date=2012-04-23 |archive-url=https://web.archive.org/web/20120423202747/http://jxb.oxfordjournals.org/content/51/345/659.full.pdf+html |url-status=live }}

The efficiency of photochemical quenching (which is a proxy of the efficiency of PSII) can be estimated by comparing $\backslash ,F\_m$ to the steady yield of fluorescence in the light $\backslash ,F\_t$ and the yield of fluorescence in the absence of photosynthetic light $\backslash ,F\_0$.

The efficiency of non-photochemical quenching is altered by various internal and external factors. Alterations in heat dissipation mean changes in $\backslash ,F\_m$. Heat dissipation cannot be totally stopped, so the yield of chlorophyll fluorescence in the absence of non-photochemical quenching cannot be measured. Therefore, researchers use a dark-adapted point ($F\_m^0$) with which to compare estimations of non-photochemical quenching.

$\backslash ,F\_0$: Minimal fluorescence (arbitrary units). Fluorescence level of dark-adapted sample when all reaction centers of the photosystem II are open.

$\backslash ,F\_m$: Maximal fluorescence (arbitrary units). Fluorescence level of dark-adapted sample when a high intensity pulse has been applied. All reaction centers of the photosystem II are closed.

$\backslash ,\{F\_0\}\text{'}$: Minimal fluorescence (arbitrary units). Fluorescence level of light-adapted sample when all reaction centers of the photosystem II are open; it is lowered with respect to $\backslash ,F\_0$ by non-photochemical quenching.

$\backslash ,\{F\_m\}\text{'}$: Maximal fluorescence (arbitrary units). Fluorescence level of light-adapted sample when a high intensity pulse has been applied. All reaction centers of the photosystem II are closed.

$\backslash ,F\_\{t\}$: Steady-state terminal fluorescence (arbitrary units). A steady-state fluorescence level decreased (= quenched) by photochemical and non-photochemical processes.

$\backslash ,T\_\{1/2\}$: Half rise time from $\backslash ,F\_0$ to $\backslash ,F\_m$.

$\backslash ,F\_v$ is variable fluorescence. Calculated as $\backslash ,F\_v$ = $\backslash ,F\_m$ - $\backslash ,F\_0$.

$\backslash tfrac\{F\_v\}\{F\_m\}$ is the ratio of variable fluorescence to maximal fluorescence. Calculated as $\backslash frac\{F\_m-F\_0\}\{F\_m\}$.{{cite journal|vauthors=Kitajima M, Butler WL |title=Quenching of chlorophyll fluorescence and primary photochemistry in chloroplasts by dibromothymoquinone.|journal=Biochim Biophys Acta|date=1975|volume=376|issue=1|pages=105–115|doi=10.1016/0005-2728(75)90209-1|pmid=1125215}} This is a measure of the maximum efficiency of PSII (the efficiency if all PSII centres were open). $\backslash tfrac\{F\_v\}\{F\_m\}$ can be used to estimate the potential efficiency of PSII by taking dark-adapted measurements.

$\backslash ,\backslash Phi\_\{PSII\}$ measures the efficiency of Photosystem II. Calculated as $\backslash ,\; Y\_\{(II)\}$ = $\backslash frac\{\{F\_m\}\text{'}-F\_t\}\{\{F\_m\}\text{'}\}$.{{cite journal|vauthors=Genty B, ((Briantais J-M)), Baker NR |title=The relationship between the quantum yield of photosynthetic electron transport and quenching of chlorophyll fluorescence.|journal=Biochim Biophys Acta|date=1989|volume=990|pages=87–92|doi=10.1016/s0304-4165(89)80016-9}} This parameter measures the proportion of light absorbed by PSII that is used in photochemistry. As such, it can give a measure of the rate of linear electron transport and so indicates overall photosynthesis.

$\backslash ,qP$ (photochemical quenching). Calculated as $\backslash ,\backslash frac\{\{F\_m\}\text{'}-F\_t\}\{\{F\_m\}\text{'}-\{F\_0\}\text{'}\}$.{{cite journal|vauthors=Schreiber U, Schliwa U, Bilger W |title=Continuous recording of photochemical and non-photochemical chlorophyll fluorescence quenching with a new type of modulation fluorometer.|journal=Photosynth Res|volume=10|issue=1–2|pages=51–62|doi=10.1007/bf00024185|pmid=24435276|year=1986|bibcode=1986PhoRe..10...51S |s2cid=23021516 }} This parameter approximates the proportion of PSII reaction centres that are open.

Whilst $\backslash ,\backslash Phi\_\{PSII\}$ gives an estimation of the efficiency, $\backslash ,qP$ and $\backslash tfrac\{F\_v\}\{F\_m\}$ tell us which processes which have altered the efficiency. Closure of reaction centers as a result of a high intensity light will alter the value of $\backslash ,qP$. Changes in the efficiency of non-photochemical quenching will alter the ratio $\backslash tfrac\{F\_v\}\{F\_m\}$.

Chlorophyll fluorescence appears to be a measure of photosynthesis, but this is an over-simplification. Fluorescence can measure the efficiency of PSII photochemistry, which can be used to estimate the rate of linear electron transport by multiplying by the light intensity. However, researchers generally mean carbon fixation when they refer to photosynthesis. Electron transport and CO₂ fixation can correlate well, but may not correlate in the field due to processes such as photorespiration, nitrogen metabolism and the Mehler reaction.

A powerful research technique is to simultaneously measure chlorophyll fluorescence and gas exchange to obtain a full picture of the response of plants to their environment. One technique is to simultaneously measure CO₂ fixation and PSII photochemistry at different light intensities, in non-photorespiratory conditions. A plot of CO₂ fixation and PSII photochemistry indicates the electron requirement per molecule CO₂ fixed. From this estimation, the extent of photorespiration may be estimated. This has been used to explore the significance of photorespiration as a photoprotective mechanism during drought.

Fluorescence analysis can also be applied to understanding the effects of low and high temperatures.

• Sobrado (2008){{cite journal|title=Leaf characteristics and diurnal variation of chlorophyll fluorescence in leaves of the 'bana' vegetation of the amazon region |year=2008 |author=Sobrado |doi=10.1007/s11099-008-0033-9 |volume=46 |issue=2 |journal=Photosynthetica |pages=202–207|s2cid=20907425 |doi-access=free }} investigated gas exchange and chlorophyll a fluorescence responses to high intensity light, of pioneer species and forest species. Midday leaf gas exchange was measured using a photosynthesis system, which measured net photosynthetic rate, gs, and intercellular CO₂ concentration ($C\_i$). In the same leaves used for gas exchange measurements, chlorophyll a fluorescence parameters (initial, $\backslash ,F\_0$; maximum, $\backslash ,F\_m$; and variable, $\backslash ,F\_v$) were measured using a fluorometer. The results showed that despite pioneer species and forest species occupying different habitats, both showed similar vulnerability to midday photoinhibition in sun-exposed leaves.

Chlorophyll fluorescence can measure most types of plant stress. Chlorophyll fluorescence can be used as a proxy of plant stress because environmental stresses, e.g. extremes of temperature, light and water availability, can reduce the ability of a plant to metabolise normally. This can mean an imbalance between the absorption of light energy by chlorophyll and the use of energy in photosynthesis.{{cite web |url=http://personalpages.manchester.ac.uk/staff/giles.johnson/default.php?page=research |title=Plant Stress Biology |publisher=Personalpages.manchester.ac.uk |access-date=2011-03-28 |archive-date=2017-07-27 |archive-url=https://web.archive.org/web/20170727171919/http://personalpages.manchester.ac.uk/staff/giles.johnson/default.php?page=research |url-status=dead }}

• Favaretto et al. (2010){{cite journal |title=Differential responses of antioxidant enzymes in pioneer and late-successional tropical tree species grown under sun and shade conditions |author=Favaretto |year=2011

|display-authors=etal |doi=10.1016/j.envexpbot.2010.06.003 |volume=70 |journal=Environmental and Experimental Botany |issue=1 |pages=20–28|bibcode=2011EnvEB..70...20F }} investigated adaptation to a strong light environment in pioneer and late successional species, grown under 100% and 10% light. Numerous parameters, including chlorophyll a fluorescence, were measured. A greater decline in $\backslash tfrac\{F\_v\}\{F\_m\}$ under full sun light in the late-successional species than in the pioneer species was observed. Overall, their results show that pioneer species perform better under high-sun light than late- successional species, suggesting that pioneer plants have more potential tolerance to photo-oxidative damage.

• Neocleous and Vasilakakis (2009){{cite journal |title=Effects of Boron and Salinity on Red Raspberry in Vitro |journal=International Journal of Fruit Science |publisher=Informaworld.com |date=2008-12-03 }} investigated the response of raspberry to boron and salt stress. An chlorophyll fluorometer was used to measure $\backslash ,F\_0$, $\backslash ,F\_m$ and $\backslash ,F\_v$. The leaf chlorophyll fluorescence was not significantly affected by NaCl concentration when B concentration was low. When B was increased, leaf chlorophyll fluorescence was reduced under saline conditions. It could be concluded that the combined effect of B and NaCl on raspberries induces a toxic effect in photochemical parameters.
• Lu and Zhang (1999) studied heat stress in wheat plants and found that temperature stability in the Photosystem II of water-stressed leaves correlates positively to the resistance in metabolism during photosynthesis.{{cite journal | last1 = Lu | first1 = Congming | last2 = Zhang | first2 = Jianhua | year = 1999| title = Effects of Water Stress on Photosystem II Photochemistry and Its Thermostability in Wheat Plants | journal = Journal of Experimental Botany | volume = 50 | issue = 336| pages = 1199–1206 | doi=10.1093/jexbot/50.336.1199| doi-access = free }}

File:Multiplex research.png

Because of the link between chlorophyll content and nitrogen content in leaves, chlorophyll fluorometers can be used to detect nitrogen deficiency in plants, by several methods.

Based on several years of research and experimentation, polyphenols can be the indicators of nitrogen status of a plant. For instance, when a plant is under optimal conditions, it favours its primary metabolism and synthesises the proteins (nitrogen molecules) containing chlorophyll, and few flavonols (carbon-based secondary compounds). On the other hand, in case of lack of nitrogen, we will observe an increased production of flavonols by the plant.{{cite journal |

title=Optically assessed contents of leaf polyphenolics and chlorophyll as indicators of nitrogen deficiency in wheat (Triticum aestivum L.) |author1=A. Cartelat |author2=Z.G. Cerovic |author3=Y. Goulas |author4=S. Meyer |author5=C. Lelarge |author6=J.-L. Prioul |author7=A. Barbottin |author8=M.-H. Jeuffroy |author9=P. Gate |author10=G. Agati |author11=I. Moya |

date=2005 |doi=10.1016/j.fcr.2004.05.002

|volume=91

|journal=Field Crops Research

|issue=1 |pages=35–49|bibcode=2005FCrRe..91...35C }}

The NBI (Nitrogen Balance Index) by Force-A, allows the assessment of nitrogen conditions of a culture by calculating the ratio between Chlorophyll and Flavonols (related to Nitrogen/Carbon allocation) .

Gitelson (1999) states, "The ratio between chlorophyll fluorescence at 735 nm and the wavelength range 700nm to 710 nm, F735/F700 was found to be linearly proportional to the chlorophyll content (with determination coefficient, r2, more than 0.95) and thus this ratio can be used as a precise indicator of chlorophyll content in plant leaves."{{cite journal|last1=Gitelson|first1=Anatoly A|last2=Buschmann|first2=Claus|last3=Lichtenthaler|first3=Hartmut K|author-link3=Hartmut K. Lichtenthaler|year=1999|title=The Chlorophyll Fluorescence Ratio F735/F700 as an Accurate Measure of the Chlorophyll Content in Plants|journal=Remote Sensing of Environment|volume=69|issue=3|pages=296–302|bibcode=1999RSEnv..69..296G|doi=10.1016/S0034-4257(99)00023-1}}

File:IMAGING-PAM Chloropyhll Fluorometer.jpg

The development of fluorometers allowed chlorophyll fluorescence analysis to become a common method in plant research. Chlorophyll fluorescence analysis has been revolutionized by the invention of the Pulse-Amplitude-Modulation (PAM) technique {{cite journal|vauthors=Schreiber U, Bilger W, Schliwa U |title=Continuous recording of photochemical and non-photochemical chlorophyll fluorescence quenching with a new type of modulation fluorometer|journal=Photosynth. Res.|date=1986|volume=10|issue=1–2|pages=51–62|doi=10.1007/bf00024185|pmid=24435276|bibcode=1986PhoRe..10...51S |s2cid=23021516 }}{{cite journal|last1=Schreiber|first1=Ulrich|title=Detection of rapid induction kinetics with a new type of high-frequency modulated chlorophyll fluorometer|journal=Photosynth. Res.|date=1986|volume=9|issue=1–2|pages=261–272|url=https://link.springer.com/chapter/10.1007/978-94-009-4412-1_24|doi=10.1007/bf00029749|pmid=24442302|bibcode=1986PhoRe...9..261S |s2cid=19087818|url-access=subscription|archive-date=2018-06-03|access-date=2017-08-28|archive-url=https://web.archive.org/web/20180603061946/https://link.springer.com/chapter/10.1007%2F978-94-009-4412-1_24|url-status=live}} and availability of the first commercial modulated chlorophyll fluorometer PAM-101 (Walz, Germany). By modulating the measuring light beam (microsecond-range pulses) and parallel detection of the excited fluorescence the relative fluorescence yield (Ft) can be determined in the presence of ambient light. Crucially, this means chlorophyll fluorescence can be measured in the field even in full sunlight.

Today, chlorophyll fluorometers are designed for measuring many different plant mechanisms. The measuring protocols: F_V/F_M and OJIP measure the efficiency of Photosystem II samples at a common and known dark adapted state. These protocols are useful in measuring many types of plant stress.{{cite book |doi=10.1007/978-1-4020-3218-9_3|isbn=978-1-4020-3217-2|chapter=Chlorophyll Fluorescence as a Probe of Photosynthetic Productivity|title=Chlorophyll a Fluorescence|series=Advances in Photosynthesis and Respiration|year=2004|last1=Baker|first1=Neil R.|last2=Oxborough|first2=Kevin|volume=19|pages=65–82}} Bernard Genty's light adapted measuring protocol ΔF/F_M’, or Y(II), is an effective and sensitive way to measure plant samples under ambient or artificial lighting conditions.{{cite journal |doi=10.1016/S0304-4165(89)80016-9|title=The relationship between the quantum yield of photosynthetic electron transport and quenching of chlorophyll fluorescence|year=1989|last1=Genty|first1=Bernard|last2=Briantais|first2=Jean-Marie|last3=Baker|first3=Neil R.|journal=Biochimica et Biophysica Acta (BBA) - General Subjects|volume=990|pages=87–92}} However, since Y(II) values also change with light intensity, one should compare samples at the same light intensity unless light stress is the focus of the measurement. Y(II) can be more sensitive to some types of plant stress than F_V/F_M, such as heat stress.{{cite journal |doi=10.1111/j.1365-3040.2004.01222.x|title=Inhibition of photosynthesis by high temperature in oak (Quercus pubescens L.) leaves grown under natural conditions closely correlates with a reversible heat-dependent reduction of the activation state of ribulose-1,5-bisphosphate carboxylase/Oxygenase|year=2004|last1=Haldimann|first1=P.|last2=Feller|first2=U.|journal=Plant, Cell and Environment|volume=27|issue=9|pages=1169–1183|doi-access=free}}

Other plant mechanism measuring protocols have also been developed. When a chloroplast absorbs light, some of the light energy goes to photochemistry, some goes to regulated heat dissipation, and some goes to unregulated heat dissipation.{{cite journal | last1 = Kramer | first1 = D. M. | last2 = Johnson | first2 = G. | last3 = Kiirats | first3 = O. | last4 = Edwards | first4 = G. | year = 2004 | title = New fluorescence parameters for determination of QA redox state and excitation energy fluxes | journal = Photosynthesis Research | volume = 79 | issue = 2| pages = 209–218 | doi=10.1023/b:pres.0000015391.99477.0d| pmid = 16228395 | s2cid = 15860339 }} Various chlorophyll fluorescence measuring parameters exist to measure all of these events. In the lake model, q_L measures photochemical quenching, Y(NYO) measures plant regulated heat dissipation, and Y(NO) measures unregulated heat dissipation. An older quenching protocol, called the puddle model, uses q_P for photochemical quenching, q_N for nonphotochemical quenching of both regulated and unregulated heat dissipation and NPQ for an estimate of nonphotochemical quenching.{{cite journal | last1 = van Kooten | first1 = O | last2 = Snel | first2 = J | year = 1990 | title = The use of chlorophyll fluorescence nomenclature in plant stress physiology | journal = Photosynth Res | volume = 25 | issue = 3| pages = 147–150 | doi=10.1007/bf00033156| pmid = 24420345 | bibcode = 1990PhoRe..25..147V | s2cid = 206766959 }} NPQ has also been resurrected to the lake model mathematically.Klughammer C., and Schreiber U. (2008) PAM Application notes 2008 1:27 -35

In addition, the parameters q_E, and pNPQ have been developed to measure the photoprotective xanthophyll cycle.{{cite journal | last1 = Muller | first1 = P. | last2 = Xiao-Ping | first2 = L. | last3 = Niyogi | first3 = K. | year = 2001 | title = Non-Photochemical Quenching. A Response to Excess Light Energy | journal = Plant Physiology | volume = 125 | issue = 4| pages = 1558–1566| doi=10.1104/pp.125.4.1558 | pmid=11299337 | pmc=1539381}}{{cite journal |doi=10.1016/j.bbabio.2012.03.026|pmid=22503831|title=Assessing the photoprotective effectiveness of non-photochemical chlorophyll fluorescence quenching: A new approach|year=2012|last1=Ruban|first1=Alexander V.|last2=Murchie|first2=Erik H.|journal=Biochimica et Biophysica Acta (BBA) - Bioenergetics|volume=1817|issue=7|pages=977–982|doi-access=free}} q_T is a measure of state transitions.{{cite journal | last1 = Ruban | first1 = A.V. | last2 = Johnson | first2 = M.P. | year = 2009 | title = Dynamics of higher plant photosystem cross-section associated with state transitions | journal = Photosynthesis Research | volume = 99 | issue = 3| pages = 173–183 | doi=10.1007/s11120-008-9387-x| pmid = 19037743 | bibcode = 2009PhoRe..99..173R | s2cid = 6194519 }} q_M is a measure of chloroplast migration,{{cite journal | last1 = Cazzaniga | first1 = S | last2 = Osto | first2 = L.D. | last3 = Kong | first3 = S-G. | last4 = Wada | first4 = M. | last5 = Bassi | first5 = R. | year = 2013 | title = Interaction between avoidance of photon absorption, excess energy dissipation and zeaxanthin synthesis against photooxidative stress in Arabidopsis | journal = The Plant Journal | volume = 76 | issue = 4| pages = 568–579 | doi = 10.1111/tpj.12314 | pmid = 24033721 | doi-access = free }} and q_I is a measure of plant photoinhibition.{{cite book |doi=10.1007/978-1-4020-3218-9_28|isbn=978-1-4020-3217-2|chapter=Light Adaptation and Senescence of the Photosynthetic Apparatus. Changes in Pigment Composition, Chlorophyll Fluorescence Parameters and Photosynthetic Activity|title=Chlorophyll a Fluorescence|series=Advances in Photosynthesis and Respiration|year=2004|last1=Lichtenthaler|first1=Hartmut K.|last2=Babani|first2=Fatbardha|volume=19|pages=713–736}}

At lower actinic light levels NPQ = qE+qT+qI

At high actinic light levels NPQ = qE+qM=qI

Some fluorometers are designed to be portable and operated in one hand.

Consistent further development into imaging fluorometers facilitate the visualization of spatial heterogeneities in photosynthetic activity of samples. These heterogeneities naturally occur in plant leaves for example during growths, various environmental stresses or pathogen infection. Thus knowledge about sample heterogeneities is important for correct interpretation of the photosynthetic performance of the plant sample. High performance imaging fluorometer systems provide options to analyze single cell/single chloroplast as well as sample areas covering whole leaves or plants.

Techniques based on the Kautsky effect do not exhaust the variety of detection and evaluation methods based on the chlorophyll fluorescence.

In particular, recent advances in the area of laser-induced fluorescence (LIF) also provide an opportunity of developing sufficiently compact and efficient sensors for

photophysiological status and biomass assessments.

Instead of measuring the evolution of the total fluorescence flux, such sensors record the spectral density of this flux excited by strong monochromatic laser light pulses of nanoseconds duration.

Requiring no 15- 20 min dark adaptation period (as is the case for the Kautsky effect methods{{cite book | title =Handy PEA: Continuous Excitation Plant Efficiency Analyser | publisher =Hansatech Instruments | date =2012 | location =Norfolk | pages =2 | url =http://www.hansatech-instruments.com/wp-content/uploads/2012/12/Handy-PEA.pdf | access-date =2014-05-23 | archive-url =https://web.archive.org/web/20160407094815/http://www.hansatech-instruments.com/wp-content/uploads/2012/12/Handy-PEA.pdf | archive-date =2016-04-07 | url-status =dead }}) and being

capable to excite the sample from considerable distance, the LIF sensors can provide fast and remote evaluation.

• Application of the LIF technique to the assessment of drought stress in cork oak (Quercus suber) and maritime pine (Pinus pinaster) on the basis of chlorophyll emission ratio I₆₈₅/I₇₄₀ is described in Ref.

{{cite journal | last =Lavrov | title = Water stress assessment of cork oak leaves and maritime pine needles based on LIF spectra

| journal =Optics and Spectroscopy | volume =112 | issue =2 | pages =271–279 | date =2012

| doi =10.1134/S0030400X12020166|display-authors=etal| bibcode = 2012OptSp.112..271L

| s2cid = 123049193

| url = https://lirias.kuleuven.be/bitstream/123456789/470333/1/UtkinSVLS101105.doc

| url-access =subscription}}

Recently the LIF sensing technique was harnessed to address the role of pPLAIIα protein in the protection of the photosynthetic metabolism during drought stress using genetically modified Arabidopsis plants.

Silvestre et al.

[http://www.sebiology.org/meetings/Past_Meetings/plant2013/programme.pdf Contribution of pPLAIIα to drought tolerance using genetically modified arabidopsis plants: II. Effects on photosynthetic metabolism.]

Int. Meeting Prog. Plant Symposium of the SEB: Oxidative stress and cell death in plants: mechanisms and implications, Florence, Italy, 26–28 June 2013, p. 5

• In 2011, Vieira et al. applied a compact low-cost LIF sensor

{{cite journal | last =Utkin | title = Compact low-cost detector for in vivo assessment of microphytobenthos using laser induced fluorescence

| journal =Optics and Spectroscopy | volume =114 | issue =3 | pages =471–477 | date =2013

| doi =10.1134/S0030400X13030259|display-authors=etal| bibcode = 2013OptSp.114..471U

| s2cid = 124095431

}}

(built around a frequency-doubled solid-state Q-switched Nd:YAG laser and a specially modified commercial miniature fiber optic spectrometer Ocean Optics USB4000) to study intertidal microphytobenthos communities. Chlorophyll emission enabled the researchers to adequately assess the surface biomass and track migratory rhythms of epipelic benthic microalgae in muddy sediments.

{{cite journal | last =Vieira | title = Effects of intertidal microphytobenthos migration on biomass determination via laser-induced fluorescence

| journal =Marine Ecology Progress Series | volume =432 | pages =45–52 | date =2011

| doi =10.3354/meps09157|display-authors=etal| doi-access =free| url =https://lirias.kuleuven.be/bitstream/123456789/470339/1/Vieira_etal_2011.pdf}}

• Integrated fluorometer for gas exchange and chlorophyll fluorescence of leaves
• Non-photochemical quenching

{{reflist|30em}}

• [http://www2.geog.ucl.ac.uk/~mdisney/teaching/GEOGG141/papers/sif.pdf Solar-induced fluorescence], geog.ucl.ac.uk
• [https://www.nutechintl.com/products/plant-research/continuous-excitation-or-prompt-chlorophyll-fluorimeters/handy-pea-advanced-continuous-excitation-chlorophyll-fluorimeter/ Advanced Continuous Excitation Chlorophyll Fluorimeter], nutechintl.com

• {{cite journal | author = Lazár | date = 1999 | title = Chlorophyll a fluorescence induction | url = https://www.researchgate.net/publication/247773250 | journal = Biochimica et Biophysica Acta (BBA) - Bioenergetics | volume = 1412 | issue = 1 | pages = 1–28 | doi=10.1016/s0005-2728(99)00047-x| pmid = 10354490 | doi-access = free }}
• {{cite journal | author = Lazár | date = 2006 | title = The polyphasic chlorophyll a fluorescence rise measured under high intensity of exciting light | url = https://www.researchgate.net/publication/247772997 | journal = Functional Plant Biology | volume = 33 | issue = 1 | pages = 9–30 | doi=10.1071/fp05095| pmid = 32689211 | s2cid = 84343023 }}
• {{cite journal | author = Lazár | date = 2015 | title = Parameters of photosynthetic energy partitioning | url = https://www.researchgate.net/publication/270646200 | journal = Journal of Plant Physiology | volume = 175 | pages = 131–147 | doi=10.1016/j.jplph.2014.10.021| pmid = 25569797 | bibcode = 2015JPPhy.175..131L }}
• {{cite journal | author = Kalaji | date = 2012 | title = Experimental in vivo measurements of light emission in plants: a perspective dedicated to David Walker |display-authors=etal | doi=10.1007/s11120-012-9780-3 | pmid = 23065335 | volume=114 | issue = 2 | journal=Photosynthesis Research | pages=69–96| bibcode = 2012PhoRe.114...69K | s2cid = 10325911 }}
• {{cite journal | doi = 10.1093/jexbot/51.345.659 | title = Chlorophyll fluorescence--a practical guide | year = 2000 | last1 = Maxwell | first1 = K. | journal = Journal of Experimental Botany | volume = 51 | issue = 345 | pages = 659–68 | pmid = 10938857 | last2 = Johnson | first2 = GN| doi-access = free }}
• {{cite journal | author = Murchie and Lawson | date = 2013 | title = Chlorophyll fluorescence analysis: a guide to good practice and understanding some new applications.| doi = 10.1093/jxb/ert208 | journal = Journal of Experimental Botany | volume = 64 | issue = 13 | pages = 3983–3998 | pmid=23913954| doi-access = }}

{{DEFAULTSORT:Chlorophyll Fluorescence}}

Category:Light reactions

Category:Photosynthesis