3.1.

Two-Photon Excitation Efficiency Measurement

In addition to comparing the fluorescence intensity excited by each laser as a function of average power, we derived a measure of 2p excitation efficiency ($\eta$) for each laser tested, as introduced in Eq. (5). Using a Ti:Sa laser, the Spectra Physics Mai Tai, as a gold standard reference and defining it to have an efficiency of $\eta =1$, the 2p excitation efficiency of each tested laser was calculated using

The repetition rate $R$ was measured by monitoring the output of a fast photodiode equipped with each laser. Each laser’s pulse duration ${\tau }_p$ was measured using an autocorrelator and assuming a ${\mathrm{sech}}^2$ pulse shape. Note that the assumption of ${\mathrm{sech}}^2$ pulse shape for reporting pulse duration is arbitrary and does not affect any of the results, which all depend on the ${\tau }_p$ ratios, but is used rather to maintain consistency with published manufacturer specifications. Values for the repetition rate and pulse duration of the Spectra Physics Mai Tai Ti:Sa reference laser, a Coherent Chameleon Ultra II Ti:Sa laser, and the four compact lasers are shown in Table 1. The normalized fluorescence intensity $F_{\text{test}}/F_{\mathrm{ref}}$ and 2p excitation efficiency $\eta$ for each laser are plotted in Figs. 2(d) and 2(e), respectively. Due to a combination of factors ($R$, ${\tau }_p$, and $\eta$), the Mai Tai Ti:Sa reference laser produced more fluorescence for the same average power than any of the compact lasers tested [Fig. 2(d)]. Once adjustments are made for the repetition rate and pulse duration, one can see that the 2p excitation efficiency varies dramatically between the various lasers. Surprisingly, the 2p excitation efficiency of the Coherent Axon 920 (mean: 1.09 ± standard deviation: 0.03) actually exceeded that of the Spectra Physics Mai Tai reference laser [$1.00\pm 0.05$, Fig. 2(e)] even though its measured (normalized) fluorescence $F_{\text{test}}/F_{\mathrm{ref}}$ ($0.57\pm 0.02$, Fig. 2(d) was modest compared to the Ti:Sa laser ($1.00\pm 0.05$), due to its long pulse duration. In contrast, the 2p excitation efficiency of the Menlo Systems YLMO laser ($0.52\pm 0.01$) was significantly worse than that of the Spectra Physics Mai Tai reference laser, reflecting in part its poor pulse quality with prominent side lobes [see green FROG trace in inset of Fig. 2(e)] compared to the Ti:Sa lasers. The fluorescence predicted from the FROG trace correlated with measured fluorescence for the few lasers where this measurement was available [inset of Fig. 2(d)], consistent with the idea that pulse shape is a factor in determining 2p excitation efficiency. It was found, however, that the FROG trace did not fully explain the variations in fluorescence observed. For the YLMO, the FROG trace overestimated the actual fluorescence by 42%, and for the Chameleon, the FROG trace overestimated the actual fluorescence by 18%, when using the Mai Tai as a reference. Thus, the more direct 2p excitation efficiency measurement carried out in this study appears to account for factors other than pulse quality as measured by FROG. Of the tested compact lasers, the Toptica Femtofiber Ultra 920 had perhaps the best combination of measured fluorescence $F_{\text{test}}/F_{\mathrm{ref}}$ ($0.75\pm 0.01$), due to its favorable repetition rate and pulse duration and 2p excitation efficiency $\eta$ ($0.86\pm 0.01$).

Table 1

Measured repetition rate and pulse duration of the Ti:Sa reference laser (Spectra Physics Mai Tai) and each tested laser. These data are shown in graphical form in Fig. S4 in the Supplementary Material.

Table 2

Computed p-values for differences between means of 2p excitation efficiency [see Fig. 2(e)] using Dunnett’s T3 multiple comparisons test.

To verify that the measured differences in 2p excitation efficiency were not due to changes in the optical system or alignment, the sizes of the excitation volumes produced by each laser were measured and compared. If the measurements of $F_{\text{test}}/F_{\mathrm{ref}}<1$ that we observed were due to aberrant foci, one would expect a negative correlation between 2p excitation efficiency and spot size across lasers. Figure 3 shows that spot sizes instead exhibited a slight positive correlation across lasers for these values ($r=0.487$ in the $x$ dimension and $r=0.677$ in the $z$ dimension) [Figs. 3(c) and 3(d)]. Thus, differences in 2p excitation between lasers could not be explained by differences in the radial or axial dimension of the laser focus. As expected, slight negative correlations are seen between 2p excitation efficiency and spot size across measurements during a single session for a given laser [see insets of Figs. 3(c) and 3(d) and Tables S1 and S2 in the Supplementary Material]. These variations for a single laser are minute, however, compared to the difference in 2p excitation efficiency between the different lasers.

Fig. 3

Differences in pulse quality cannot be explained by variation in laser spot size. Measurements of the FWHM of the excitation volume in the (a) lateral and (b) axial dimensions for each laser across six different power levels are shown below representative excitation volume images. Note that the same set of images is used in both panels (a) and (b). Error bars indicate standard deviation. (c), (d) 2p excitation efficiency [see Eq. (6), Fig. 2(e)] is not dependent on the size of the excitation volume. Different shading and numbering are used to denote multiple data-collection sessions on different days with laser realignment in between (three sessions for the Mai Tai; 2 for the YLMO, Axon, and Alcor; and 1 for the Chameleon and FF Ultra). (c) Radial and (d) axial spot dimensions exhibited a slight positive correlation with 2p excitation efficiency across different lasers and sessions ($r_{\text{radial}}=0.487$ and $r_{\text{axial}}=0.677$, respectively). Slight negative correlations are seen across the vast majority of single data-collection sessions, with examples shown in insets. All single session correlation coefficients are provided in Tables S1 and S2 in the Supplementary Material.

5.1.

Cuvette Design and Assembly

To measure 2p fluorescence efficiency, a custom stainless steel cuvette filled with $10\mu \text{M}$ Atto 488 dye and capped with a No. 1 cover glass was constructed in a manner such that no air gap between the cover glass and the solution was introduced [see Fig. 1(l); Code, Data, and Materials Availability section for computer-aided design (CAD) files and drawings]. The cuvette was comprised of a $10\mathrm{mm}\times 10\mathrm{mm}\times 12.5\mathrm{mm}$ stainless steel block with Ø 9 mm holes bored into the top and side to form the cavity for the solution and to form the excitation and viewing windows. A Unified National Fine (UNF) 1/4-28 threaded hole was formed in the bottom for mating with the base. Two $10\mathrm{mm}\times 10\mathrm{mm}$ squares were cut from No. 1 cover glass using a diamond scribe. The pieces of cover glass were bonded to the excitation and viewing windows with optical adhesive (Norland Products NOA 81) and cured using ultraviolet (UV) light. The base of the cuvette was comprised of a $10\mathrm{mm}\times 10\mathrm{mm}\times 15\mathrm{mm}$ stainless steel block with a protruding UNF 1/4-28 threaded rod for mating with the cuvette. A size $-008$ soft Viton O-ring (McMaster-Carr 1284N108) was slipped over the rod to ensure a watertight seal when screwed into the threaded hole of the cuvette. A Unified National Coarse (UNC) 8-32 threaded hole was formed in the bottom face of the base, opposite the rod, for mating to a standard 1/2″ optical post (e.g., Thorlabs TR series).

To fill the cuvette, it was inverted and slightly overfilled with $10\mu \text{M}$ Atto 488 solution using a transfer pipette. The cuvette base was then carefully but tightly threaded into the cuvette, ensuring minimal formation of air bubbles. The filled cuvette was stored in an inverted position between experiments to prevent the migration of air bubbles to the excitation window.

5.2.

Measurement of Generated Fluorescence

The beams of the reference laser (Spectra Physics Mai Tai HP with DeepSee), the second Ti:Sa laser (Coherent Chameleon Ultra II), and each of the four compact lasers (Toptica Femtofiber Ultra 920, Coherent Axon 920, Menlo Systems YLMO 930, and Spark Alcor 920-2) were expanded and collimated, using a pair of achromatic doublet lenses and a standard 2p microscope scan lens (Thorlabs SL50-2P2) and tube lens (Thorlabs TTL200MP), to just overfill a water immersion microscope objective (Nikon CFI75 LWD 16X W). The objective was lowered into a drop of water on the cuvette’s coverslip to focus the beam into the dye and generate a volume of excited fluorescence. Fluorescence was imaged onto a camera (FLIR BFLY-PGE-31S4M-C) through a No. 1 cover glass window on the side of the cuvette using a long working distance objective (Mitutoyo Plano Apo Infinity Corrected LWD 20X) and an $f=200\mathrm{mm}$ achromatic doublet tube lens (Thorlabs AC254-200-A). An IR-blocking filter was placed in front of the camera to block out laser light. Except for the Chameleon Ultra II Ti:Sa laser, which does not have a group delay dispersion (GDD) compensator, each laser’s built-in GDD compensator was tuned until the highest single pixel value in the image was maximized. See Fig. 1(k) for the schematic.

Each laser tested was manually swapped and aligned into the optical system. The same laser was sometimes realigned multiple times for multiple imaging sessions [see Figs. 3(c) and 3(d)]. Because the different compact lasers were tested in some cases several months apart, the fluorescence measurement with the Mai Tai Ti:Sa reference laser was repeated whenever a new subset of the compact lasers was measured to verify the stability of the fluorescence from the cuvette over time (see Fig. S2 in the Supplementary Material).

5.3.

Image Capture and Normalization

For each image of the excitation volume taken, the camera exposure was adjusted in the range of 600 ms to 5 s so that the intensity of the brightest pixel was maximized without saturating. This resulted in different exposure levels across different lasers and different power levels. Each image was stored as a matrix of 16-bit unsigned integers (12-bit pixel depth scaled to 16 bits). To normalize images with different exposure levels for direct comparison, each image was first converted to double precision. Then the mean value of the background was calculated and subtracted from the image. Finally, the new image was divided by the exposure value in milliseconds. The linearity of the camera and this conversion was confirmed by imaging the same fluorescent spot with a series of different exposure times (Fig. S1 in the Supplementary Material). The value of the brightest pixel in each resulting image was used to quantify intensity. The excitation volume profile measurements were taken along the row and column of the brightest pixel in each image. Image processing and calculations were performed using custom routines in MATLAB.

To compute values for normalized fluorescence [plotted in Fig. 2(d)], every data point across all lasers and all power levels was divided by the fluorescence value predicted by the log–log regression of the Mai Tai at the same amount of laser power. This allows for comparison of fluorescence from each laser independent of power level and brings the average value of fluorescence from the Mai Tai reference laser to 1, facilitating the calculation of fluorescence ratios between lasers.

5.4.

Pulse Duration and Repetition Rate Measurements

For each laser, except the Coherent Chameleon Ultra II, a small fraction of the beam intensity exiting the laser head was reflected using a cover glass and directed into an autocorrelator (APE Mini PD). A 1.5 ps scan length was used in FRINGES mode with an averaging factor of 8 and smoothing turned off. Sensitivity and gain were adjusted to achieve high dynamic range without saturating. The autocorrelator calculated the pulse duration from the autocorrelation trace by measuring the width of the ACF when it decays to ½ its amplitude (autocorrelation time) and dividing the value by the deconvolution factor for a ${\mathrm{sech}}^2$ pulse (1.54). Each laser’s group delay dispersion compensator was adjusted until the peak on the autocorrelator display was maximized and the displayed pulse duration was minimized. The reported pulse duration was then recorded.

The pulse width of the Coherent Chameleon Ultra II was measured using an FROG device (Swamp Optics GRENOUILLE 10-100-USB). Because there is no GDD compensation on the Chameleon, the beam was sent into the device after being propagated through the optical system used for fluorescence measurements (see Sec. 5.5 for details) to maintain a consistent GDD between fluorescence and pulse width measurements. To remain consistent with the pulse width measurements for the other lasers, the pulse width of the Chameleon Ultra II was calculated using the FROG device’s autocorrelation measurement and dividing by the ${\mathrm{sech}}^2$ deconvolution factor of 1.54.

Each laser came equipped with a fast photodiode placed in the path of a reflected portion of the beam. To measure the repetition rate of each laser, its photodiode output was connected to a digital oscilloscope (Tektronix TDS1001B), which automatically calculated the frequency of the recorded trace.

5.5.

FROG Measurements and Calculations

FROG measurements were performed on a subset of the lasers tested in this study (Spectra Physics Mai Tai, Coherent Chameleon Ultra II, and Menlo Systems YLMO 930) to compare actual fluorescence measurements to the fluorescence predicted by the pulse shape and duration. To capture the effects of GDD and each laser’s built-in GDD compensation (or lack thereof in the case of the Chameleon) on the pulse, the laser beam was sent into a FROG device (Swamp Optics GRENOUILLE 10-100-USB) after being propagated through the simple microscope optical system [Fig. 1(k)]. Because the device requires a collimated input beam, the convergent beam exiting the microscope objective was first collimated with a 0.83 NA aspheric lens (Edmund Optics 67-257) before being coupled into the FROG device. Note that the water immersion normally used with the Nikon 16× objective was not used in the FROG measurements. To keep the beam at a reasonable diameter ($\sim 4\mathrm{mm}$) for the FROG device and avoid aberrations, the two initial achromatic doublets in the system were switched for achromatic doublets with different focal lengths to reduce the initial beam magnification and underfill the microscope objective. While this greatly lowered the effective NA of the microscope objective, swapping the achromatic doublets and adding the aspheric lens had minimal effect on the overall GDD of the system.

The normalized fluorescence (described in paragraph 2 of Sec. 5.3) was plotted against the fluorescence ratio predicted by FROG [see inset of Fig. 2(d)]. The FROG-predicted fluorescence ratio was calculated directly from the FROG pulse trace, which is independent of laser power and has an amplitude of 1 in arbitrary units. First, a constant laser power level of 1 W was assumed to simplify calculations. The FROG pulse trace was integrated using trapezoidal sums. Every point in the pulse trace was then divided by this integral and multiplied by the pulse energy for that laser at 1 W (1 W divided by the repetition rate) to yield a pulse trace with an integral equal to the energy of a single pulse at 1W average power. Then this power-normalized pulse trace was squared and integrated using trapezoidal sums, and this value was multiplied by the laser repetition rate to yield a value for the predicted 2p fluorescence of each laser, as in Eq. (1). Finally, this predicted value for each laser was normalized to the corresponding value for the Mai Tai reference laser to yield the FROG-predicted fluorescence ratio. See Fig. S3 in the Supplementary Material inset for representative FROG pulse traces from each of the lasers measured.

5.6.

Wavelength Dependence of Fluorescence

All of the compact 2p lasers tested have a nominal peak wavelength of 920 nm, except for the Menlo Systems YLMO 930, which has a peak wavelength of 930 nm. To ensure that this difference in wavelength would not affect the amount of excited fluorescence and the calculated pulse quality, the methods in Secs. 5.1–5.4 were repeated with the Mai Tai Ti:Sa laser tuned between 920 and 930 nm. The fluorescence intensity was measured at each location and normalized by the pulse width at each location to isolate the wavelength dependence of 2p excitation efficiency of the Atto 488 dye. There was no significant difference in fluorescence intensity generated among the different wavelengths [One-way analysis of variance (ANOVA), $p=0.26$, see Fig. S3 in the Supplementary Material].